Isolation and molecular characterisation of flavonoid 3′-hydroxylase
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ISOLATION AND
CHARACTERISATION OF A NOVEL
GLYCOSAMINOGLYCAN
WITH ANTICANCER ACTIVITY
Olanrewaju D Ogundipe
School of Environmental and Life Sciences
University of Salford, Salford, UK
Submitted in Partial Fulfilment of the
Requirements of the Degree of Doctor of Philosophy,
May, 2015
ii
Contents ii
List of figures xi
List of tables xvi
Abbreviations xviii
Acknowledgements xxiv
Abstract xxvi
Section 1: Introduction and overall aim of this study 1
1.0 General introduction 2
1.1 Glycosaminoglycans 7
1.2 GAG’s structure and functions 10
1.3 Heparin /HS structures and functions 11
1.4 CS/DS structures and functions 13
1.5 Glycosaminoglycans isolated from shellfish 17
1.6 Biosynthesis of GAGs 17
1.7 Biosynthetic modification of HS- GAGs chain 21
1.8 Biosynthetic modifications CS/DS- GAGs chain 23
1.9 Analysis of GAGs and their oligosaccharides
fragments
25
1.10 Traditional methods for extraction and purification
of GAGs from Tissue Samples and Cultured Cells
25
1.11 Chemical and enzymatic depolymerisation of
GAGs used in structural analysis
26
iii
1.12 Use of separations techniques for structural
analysis
28
1.13 Strong anion-exchange chromatography
(SAX-HPLC)
29
1.14 Polyacrylamide gel Electrophoresis (PAGE) 30
1.15 GAG’s degrading enzymes 30
1.16 Heparinases 31
1.17 Heparinase I from F. heparinum (EC 4.2.2.7) 33
1.18 Heparinase 11 from F. heparinum 34
1.19 Heparinase III from f. Heparinum (E.C 4.2.2.8) 35
1.20 Chondroitinases 36
1.21 Glycosaminoglycans and cancer 39
1.22 Tumour angiogenesis 42
1.23 Fibroblast growth factors receptors (FGFRs)
in human breast cancer
47
1.24 The cell cycle 49
1.25 Cell Cycle regulation 52
1.26 Role of cell cycle regulatory molecules in Breast
Cancer Development and Progression
53
1.27 Cyclin D1 54
1.28 Cyclin E1 56
1.29 p27 and p21 56
1.30 Therapeutic target in breast cancer 57
iv
1.31 Modulation of the cell cycle 58
1.32 Direct inactivation of checkpoint controls 60
1.33 Cell death 63
1.34 Necrosis 63
1.35 Pathophysiology and physiological factors
leading to necrosis
64
1.36 Apoptosis 65
1.37 Morphology of Apoptosis 70
1.38 Biochemical features of apoptosis 73
1.39 Activation of caspases 73
1.40 DNA fragmentation 76
1.41 Phosphatidylserine (PS) Translocation 76
1.42 Mechanism of apoptosis 77
1.43 Extrinsic Pathway (caspace -8 apoptosis) 80
1.44 Intrinsic Pathway (mitochondria apoptosis) 81
1.45 Perforin/granzyme Pathway 82
1.46 Execution Pathway 84
1.47 Importance of Apoptosis 86
1.48 Apoptosis and necrosis: compare and contrast 87
1.49 Apoptosis and cancer 90
1.50 GAG’s and apoptosis 91
1.51 Overall aims of this study 92
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Section 2: Experimental Materials and Methods 95
2.0 Experimental Materials 96
2.1 Methods 98
2.2 Preparation of GAGs 98
2.3 Desalting of Crude GAGs 99
2.4 Purification of crude GAGs by anion-exchange
chromatography
99
2.5 Desalting of purified GAGs fractions 99
2.6 Enzyme digestion of GAGs 100
2.7 Chemical treatment (nitrous acid treatment) 100
2.8 Polyacrylamide gel electrophoresis (PAGE) analysis) 100
2.9 Superose-12 size exclusion chromatography 101
2.10 Cellulose acetate dot blotting of GAGs 102
2.11 Gel Filtration (TSK G2000 SW Column) 102
2.12 Disaccharide analysis of GAG chain by strong
anion-exchange high` Performance liquid
chromatography (SAX-HPLC)
102
2.13 Determination of cells viability (MTT assay). 103
2.14 Flow Cytometry Analyses of DNA Content
(Cell cycle analysis)
104
2.15 Annexin V-FITC apoptosis detection 105
2.16 DAPI fluorescent microscopy for apoptosis detection 105
2.17 Statistical Analysis 106
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Section 3: Results 107
3.0 Biological evaluation of cockle derived
GAG mixtures
108
3.1 Effects of cockle derived GAG mixtures on
MDA468 breast cancer cell growth
(MTT assay results)
108
3.2 Effects of Cockle derived GAG mixtures
on the MDANQ01 breast cancer cell
110
3.3 Effect of crude cockle GAG mixture on
human lymphoblastic leukaemia (MOLT-4)
cell proliferation in vitro
112
3.4 Effects of crude cockle GAG mixtures on t
he growth of K562 erythroleukaemia cells in vitro.
114
3.5 Effect of cockle GAG mixtures on 3T3 normal
fibroblast cell line
116
3.6 Cell cycle analysis of the MOLT-4 cell line
after treatment with cockle GAG extracts
118
3.7 Annexin V-FITC Apoptosis Assay of the MOLT-4
Lymphoblastic leukaemia cell line following treatment
with crude cockle GAG
124
Section 3B: Biological assay results for whelk GAG mixture 128
3.8 Effect of crude whelk GAG extracts on growth of the
MDANQ01 breast cancer cell line
129
3.9 Effect of crude whelk GAG extracts on the
growth of MDA468 breast cancer cells
131
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3.10 Effect of crude whelk GAG extracts on the
growth of K562 and MOLT-4 leukaemia cells
lines (K562 and MOLT-4)
133
3.11 Effect of crude whelk GAG extracts on growth of
HeLa Cervical cells
135
3.12 Effect of crude whelk GAG mixtures on
the growth of normal fibroblast cells (3T3)
137
3.13 Effect of Heparinase I, II, & III enzymes on
anti-proliferative activity of whelk GAG mixtures
using MDA468 and MDANQ01 breast cancer cell lines.
139
3.14 Cell cycle analysis of MDANQ01 cells after
treatment with crude whelk GAG extracts
141
3.15 Cell cycle analysis of MDA468 breast cancer cell
lines after treatment with crude whelk GAG extracts
144
3.16 Effects of crude whelk GAG mixtures on the
induction of apoptosis in MDA468 breast cancer cells
147
3.17 Flow cytometry and Annexin V-FITC detection of
MDANQ01 cells following incubation with whelk
GAG extracts
151
3.18 Assessment of apoptosis using DAPI fluorescent
microscopy following treatment of MDA468
breast cancer cell with Crude whelk GAG extracts
154
3.19 Assessment of apoptosis using DAPI fluorescent
microscopy following treatment of MDANQ01 breast
cancer cell with Crude whelk GAG
156
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3.20 Assessment of apoptosis using annexin V-FITC apoptosis
detection following treatment of HELA cells with crude
whelk GAG extracts
159
3.21 Assessment of apoptosis using DAPI microscopy
treatment of HELA cells with whelk GAGs
161
3.22 Fractionation of whelk GAG extracts by
ion-exchange chromatography
164
Section 3C: Biological activities of purified whelk fraction E 168
3.23 Effect of purified whelk fraction E on the growth
of MDANQ01 breast cancer cells
169
3.24 Effect of purified whelk fraction E on MDA468 171
breast cancer cell proliferation
3.25 Cell cycle analysis of the MDANQ1 breast cancer
cell line after treatment with purified whelk fraction E
173
3.26 Cell cycle analysis of the MDA468 cell line after
treatment with Purified whelk fraction E
175
3.27 Purified whelk fraction E induces mild apoptosis
and necrosis on MDANQ01 breast cancer cells
(revised Annexin V-FITC apoptosis detection
assay results).
178
3.28 Annexin V-FITC apoptosis assay of the MDA468
breast cancer cell line following treatment with
purified whelk fraction E
180
Section 3D: Characterisation and purification assay results for cockle GAGs 184
3.29 Assignment of unsaturated CS disaccharides from 185
cockle GAG extracts.
3.30 Assignment of unsaturated HS dissacharides from 188
cockle GAG extracts
ix
3.31 Gel Filtration analysis (TSK 2000PW) of heparinase 191
degraded cockle GAG extracts
3.32 Superose 12 size exclusion chromatography 193
analysis of intact cockle extracted GAG chains
3.33 PAGE analysis of crude cockle GAG extracts 195
and commercial GAGs after enzymatic
depolymerisation.
Section 3E: Characterisation of crude whelk GAG mixtures 197
3.34 Assignment of unsaturated CS disaccharides 198
for whelk GAG extracts
3.35 PAGE analysis of crude whelk GAG extracts 202
and commercial GAGs after enzymatic
depolymerisation
3.36 Superose-12 size exclusion chromatography of 204
crude whelk GAG extracts.
Section 3F: Characterisation of purified whelk GAG fractions 206
3.37 Assignment of unsaturated CS disaccharides 207
from purified whelk GAG fractions
3.38 Heparinase I-III enzymatic treatments and
disaccharide analysis by SAX-HPLC of the 210
active whelk fraction E
3.39 HPLC Gel Filtration analysis of whelk 214
fraction E after heparinase degradation
x
3.40 PAGE analysis of purified whelk fractions 216
and commercial GAGs after enzymatic
depolymerisation
3.41 Superose-12 size exclusion chromatography 218
of purified whelk fraction E
Section 4: Discussion 220
4.1 Outline of the major findings 221
4.2 Selective anti-cancer activity of cockle
GAGs against leukemia cell lines
223
4.3 Evidence of broader and stronger anti-cancer
activity of whelk GAGs extracts
224
4.4 Selective anti-cancer activity of whelk
bioactive fraction E against breast cancer cell
227
4.5 Molecular mechanism of action of cockle
GAG extracts on leukaemia cell lines
228
4.6 Molecular mechanism of action of whelk
GAG extracts on breast cancer cell
231
4.7 Cockle GAG mixture inhibit proliferation
of MOLT-4 leukaemia cell partly by apoptosis
233
4.8 Crude and purified whelk GAG extracts inhibit
cancer cell growth by apoptosis, analysis by
annexin V staining
235
4.9 PAGE and size exclusion analysis of cockle
GAG mixture
236
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4.10 SAX-HPLC and gel-filtration of cockle GAG
extracts
238
4.11 Ion- exchange fractionation of crude whelk
GAG mixture
243
4.12 PAGE and size exclusion analysis of both
crude and ion-exchange purified whelk GAG
extracts
244
4.13 SAX-HPLC and gel-filtration of whelk GAGs 246
4.14 SAX-HPLC and gel-filtration of whelk
bioactive fraction E
248
4.15 Overall summary 254
4.16
4.16
Limitation of this study
Future direction
References
255
256
257
List of Figures
Figure 1.1 Schematic structures of GAGs. 9
Figure 1.2 Structure of different types of CS 16
Figure 1.3 Schema of the biosynthetic assembly
of the GAG backbones by various glycosyltransferases.
20
Figure 1.4 HS chain elongation 22
Figure 1.5 Pathways of CS/DS chain elongation 24
Figure 1.6 Primary glycosidic linkages cleaved by Heparin lyases 32
Figure 1.7 Unsaturated disaccharides derived from HS by 34
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enzyme catalysed elimination
Figure 1.8 Glycosidic linkages cleaved by chondroitin lyases 37
Figure 1.9 Unsaturated disaccharides derived from chondroitin
sulfate by enzyme catalysed elimination
38
Figure 1.10 Stages involves in tumour angiogenesis 46
Figure 1.11 The cell cycle showing the two major events that takes place
within the cell
49
Figure 1.12 The four stages of mitosis 51
Figure 1.13 The cell cycle and its regulation by cyclins,
CDKs, and CDKIs
52
Figure 1.14 The processes involved in apoptosis 66
Figure 1.15 Stages of apoptosis 69
Figure 1.16 Morphology of apoptosis 71
Figure 1.17
Figure 1.18
Figure 1.19
Figure 3.1
Activation of apoptosis signaling pathway
Intrinsic and extrinsic pathway
Differences between apoptosis and necrosis
MTT cell viability assay for MDA468 cells
after treatment with cockle derived and
commercially sourced GAG chains
75
79
89
109
Figure 3.2 MTT cell viability assay for MDANQ01
cells after treatment with cockle derived
and commercially sourced GAG chains
111
Figure 3.3 MTT cell viability assay for MOLT-4
lymphoblastic leukaemia cells after treatment
with cockle derived and commercially sourced
113
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GAG chains
Figure 3.4 Concentration-dependent effect of Cockle GAG
mixtures on K562 erythroleukaemia cell viability
115
Figure 3.5 MTT cell viability assay for normal fibroblast (3T3)
cells after treatment with cockle GAGs
117
Figure 3.6 (i) Cell cycle analysis of MOLT-4 lymphoblastic
leukaemia cell line following treatment with
50µg/ml of cockle GAG extracts
119
Figure 3.6 (ii) Cell cycle analysis of MOLT-4 lymphoblastic
leukaemia cell line following treatment with low
concentration (20µg/ml) of cockle GAG extract.
123
Figure 3.7 Detection of Apoptotic MOLT-4 cells treated
with cockle GAG by Annexin V Staining.
126
Figure 3.8 MTT cell viability assay for MDANQ01 cells
after treatment with Whelk extract and
commercial GAGs
130
Figure 3.9 Concentration-dependent effect of whelk GAG
extracts on MDA468 breast cancer cell viability
132
Figure 3.10 MTT cell viability assay for MOLT-4 and K562
leukaemia cells after treatment with whelk GAG
extracts
134
Figure 3.11 MTT cell viability assay for HELA cervical cell
after treatment whelk GAG extracts
136
Figure 3.12 MTT cell viability assay of normal fibroblast 3T3
cells after treatment with whelk GAGs extracts
138
Figure 3.13 MTT cell viability assay for MDANQ01 and
MDA468 breast cancer cells after treatment with
140
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heparinase depolymerised whelk GAG extracts
Figure 3.14 Cell cycle analysis of MDANQ01 breast cancer cell line following
treatment with crude whelk GAG extract
142
Figure 3.15 Cell cycle analysis of MDA468 breast cancer cell line following
treatment with crude whelk GAG extract
145
Figure 3.16 Detection of Apoptotic MDA468 breast cancer cells
treated with crude whelk GAG extracts by Annexin
V Staining
149
Figure 3.17 Detection of Apoptotic MDANQ01 breast cancer
cells treated with crude whelk GAG extracts by
Annexin V Staining
152
Figure 3.18 Detection of apoptotic MDA468 cells by DAPI
fluorescent microscopy following treatment
with crude whelk GAG extracts
155
Figure 3.19 Detection of apoptotic MDANQ01 cells
treated with crude whelk GAG mixtures
by DAPI fluorescent microscopy
157
Figure 3.20 Detection of Apoptosis in HELA cells by Annexin
V Staining following treatment with whelk GAG
extracts
160
Figure 3.21 Detection of apoptotic HELA cells by DAPI
fluorescent microscopy following treatment
with whelk GAG
162
Figure 3.22 Ion-exchange chromatography elution profile for
whelk GAG extracts
165
Figure 3.23 MTT cell viability assay for MDANQ01 breast
cancer cells after treatment with GAG mixtures
170
xv
and purified fraction E
Figure 3.24 Concentration-dependent effect of purified whelk
GAG fraction E on MDA468 breast cancer cell viability
172
Figure 3.25 Cell cycle analysis of MDA468 breast cancer cell line following
treatment with purified whelk fraction E
174
Figure 3.26 Detection of Apoptotic MDANQ01 breast cancer cells
treated with purified whelk fraction E by Annexin V
Staining
176
Figure 3.27 Detection of Apoptotic MDANQ01 breast cancer
cells treated with purified whelk fraction E by Annexin V Staining
179
Figure 3.28 Detection of time-dependent Apoptotic MDA468
breast cancer cells treated with purified whelk
fraction E by Annexin V Staining
181
Figure 3.29 Kinectic of chondroitinase ABC enzyme degradation of
commercial CS
187
Figure 3.30 Analytical TSK2000PW gel-filtration profiles of
HS/Heparin and crude cockle GAGs after complete
digestion with Heparinase I, II and III enzymes
193
Figure 3.31 Superose 12 size exclusion chromatography and cellulose
acetate dot blotting result for crude cockle GAG mixture
194
Figure 3.32 PAGE analysis of enzymatic depolymerised GAGs. 196
Figure 3.33 Kinetic of chondroitinase ABC enzyme degradation
of GAGs
199
Figure 3.34 PAGE analysis of enzymatic depolymerised GAGs 203
Figure 3.35 Superose 12 size exclusion chromatography and cellulose
acetate dot blotting assay of crude whelk GAG extract
205
xvi
Figure 3.36 Analytical TSK2000PW gel-filtration profiles of HS/heparin
and purified whelk fraction E after complete digestion with
Heparinase I, II and III enzymes
215
Figure 3.37 PAGE analyses of enzymatic depolymerised whelk
derived and commercial GAGs.
217
Figure 3.38 Superose-12 size exclusion chromatography and cellulose
acetate dot blotting assay for purified fraction E GAG mixtures
219
List of tables
Table 1
Table 2
Summary of biological effect of cockle GAGs
Ion-exchange chromatographic separation of
whelk GAG mixtures
127
158
Table 3
Table 4
Table 5
Summary of biological effect of whelk GAG
Summary of biological effect of fraction E
Disaccharides compositions of CS/DS-like
glycans found in cockle GAG mixtures
167
183
186
Table 6 HS Disaccharides compositions from
heparinase digest of cockle GAG extracts
190
Table 7 Disaccharides compositions of CS/DS-like
glycans found in whelk GAG mixtures
201
Table 8 Disaccharides compositions of CS/DS-like
GAGs present in ion-exchange purified whelk
peaks B and C
209
xvii
Table 9 Disaccharides compositions of HS-like GAGs
found in purified whelk fraction E
212
Table 10 Disaccharides compositions of HS-like GAGs 213
found in purified 204 whelk fraction E depolymerised
by heparinase III lyase
xviii
Abbreviations
∆
delta
µg
microgram
µl
Microlitre
2-OST
2-O sulfotransferase
3-OST
3-O sulfotransferase
6-OST
6-O sulfotransferase
aFGF
acidic fibroblast growth factor
AIF
Apoptosis Inducing Factor
AKT
Protein kinase B
Ala
Alanine
ANOVA
Analysis of variance
Apo2L/DR
Apo2 ligand/ Death receptor
Apo3L
Apo3 ligand
APS
Ammonium Per Sulfate
AS
Acharan sulfate
ATIII
Antithrombin III
ATP
Adenosine triphosphate
Bax
BCL2 associated X protein
Bcl-2
B-cell lymphoma protein 2
bFGF
basic fibroblast growth factor
C4ST
Chondroitin 4- O –sulfotransferase
C6ST
Chondroitin 6- O –sulfotransferase
Ca2+
Calcium ion
CaCl2
Calcium Chloride
CAD
Caspase-Activated DNAse
Caspace
Cysteinyl aspartic acid-protease
CD36
Cluster of differentiation 36
CD8+
Cluster of differentiation8+
CDK
cyclin dependent kinase
CDKI
cyclin dependent inhibitors
CE
capillary electrophoresis
xix
ChPF
Chondroitin polymerizing factor.
ChSy
Chondroitin synthase
COO-
Carbonic acid
CPD
cetylpyridinium chloride
CS
Chondroitin sulfate
CS GlcAT-II
Chondroitin sulfate GlcA transferase-II
CS/DS2ST
uronyl 2- O –sulfotransferase
CTLs
Cytotoxic T lymphocytes
CZE
Capillary zone electrophoresis
D4ST
Dermatan 4- O –sulfotransferase
DAPI
4',6-diamidino-2-phenylindole
DEAE
Diethylaminoethyl
DIABLO
Direct IAP binding protein with low PI
DISC
Death-inducing signalling complex
DMSO
Dimethyl sulfoxide
DNA
Deoxyribonucleic acid
dp
Degree of polymerization
dp10
decasaccharides
dp2
disaccharides
dp4
tetrasaccharides
dp6
hexasaccharides
dp8
octasaccharides
DR
Death receptor
DS
Dermatan sulfate
ECM
Extracellular matrix
EDAC
1-ethyl-3-(3-dimethylaminopropyl) carbodiimide
EDTA
Ethylenediaminetetraacetic acid.
ER
Eostrogen receptor
ER-ve
Eostrogen receptor negative
ER+ve
Eostrogen receptor positive
EXT
Exostosin glycosyltransferase
FADD
Fas-associated death domain
Fas
Fatty acid synthetase
xx
FasL
Fatty acid synthetase ligand
FasL/ FasR
Fatty acid synthetase ligand /Fatty acid synthetase receptor
FasR
Fatty acid synthetase receptor
FCS
fetal calf serum
FGF
Fibroblast growth factors
FGFR’s
Fibroblast growth factors receptors
FITC
Flourescein isothiocyanate
FPLC
Fast Protein Liquid Chromatography
G1
Gap 1
G2
Gap 2
GAG-PG
Glycosaminoglycans proteoglycans
GAGs
Glycosaminoglycans/Galactosaminoglycans
Gal
Galactose
GalNAc
N-acetyl galactosamine
Gal-NAc4S-
6ST
GalNAc 4-sulfate 6- O –sulfotransferase
GalNAcT,
GalNAc transferase
GalT
β4-galactosyl transferase
G-CSF
Follistatin Granulocyte colony-stimulating factors
GlcA
Glucuronic acid
GlcAT
β3-GlcA transferase
GlcNAc
N-acetyl glucosamine
GlcNAc(6S)
6-O-sulfated N-acetylglucosamine
GlcNS
N-sulfoglucosamine
GlcNS(6S)
6-O-sulfated N-sulphoglucosamine
GlcUA
β-D-glucuronic acid
Gly
Glycine
HA
Hyaluronic acid
HCG
Human chorionic gonadotropin
HCl
Hydrochloride acid
HEPES
2-[4-(2-hydroxyethyl)piperazin-1-yl]ethanesulfonic acid
HGF
Hepatocyte growth factor
HS
Heparan sulfate
xxi
HS-GAGs
Heparan sulfate glycosaminoglycans
HSPG
Heparan sulfate proteoglycans
IAP
inhibitors of apoptosis proteins
IC50
half maximal inhibitory concentration
ICAD
Inhibitor of Caspase Activated DNAse
IdoA
Iduronic acid
IdoA (2S)
2-O-sulfated IdoA
IdoUA
α-L-iduronic acid
Ig
immunoglobulin-like
Kb
kilo bytes
kDa
Kilodalton
KS
Keratan sulfate
LDL
low density lipoprotein
L-IdoA
L- iduronic acid
M
Mitosis
Mg2+
Magnesium Ion
ML
Millilitre
mM
millimolar
MOPS
3(n-Morpholino) Propanesulfonic acid
MPT
mitochondrial permeability transition
MTT
3-(4,5-Dimethylthiazol-2-yl)-2,5-Diphenyltetrazolium Bromide
NDST
N-deacetylase, N-sulfotransferase
nm
nanometre
NO
Nitric oxide
NuMA
Nuclear mitotic apparatus protein
O-Ser
O Serine
PAGE
polyacrylamide gel electrophoresis
PAP
3ˈPhosphoadenosine 5ˈphosphosulfate
PARP
Poly (ADP-ribose) polymerase
PBS
Phosphate Buffer Saline
PI
propidium iodide
xxii
pRB
retinoblastoma gene products
Procaspase-8
Pro cysteinyl aspartic acid-protease 8
Rb
Retinoblastoma
RIP
Receptor-interacting protein
ROS
Reactive oxygen species
Rpm
Rotation Per Minute
RPMI
Roswell Park Memorial Institute
Rt
retention time
RTKs
receptor tyrosine kinases
S
Synthesis
SDS-PAGE
sodium dodecyl sulfate-polacrylamide gel electrophoresis
SEM
Standard Error of Mean
Ser
Serine
SGBS
Simpson–Golabi–Behmel syndrome
SMAC
Second mitochondrial activator of caspase
SNPs
Single nucleotide polymorphisms
SO3
Sulfur trioxide
SRC
Steroid receptor coactivator
TEMED
N,N,N’,N’-Tetramethylethylendiamine
TGF-β
tumour growth factor beta
Th2
Type 2 helper
TK
Tyrosine kinase
TKR’s
Tyrosine kinase receptors
TNF
tumour necrosis factor
TNFR1
Tumour necrosis factor receptor
TNF-α
tumour necrosis factor alpha
TRADD
TNF receptor-associated death domain
Tris
Trizma base
UCN-01
7-hydroxystaurosporine
UDP
Uridine diphosphate
UV
Ultraviolet
V0
Void volume
VEGF
Vascular endothelial growth factor
xxiii
Vt
Final volume
Xyl
Xylose
xxiv
Acknowledgement
I dedicate this thesis to God almighty and the three special people in my life: my husband and
our twins, David and Esther. Thank you for your support and understanding. I would like to
thank my parents and my in-laws for their prayers and support over the past four years.
My sincere appreciation is also extended to Dr Jeremy Allen, Dr Lucy Smith, Helen
and Ross for their support and training in flourescent microscopy. Jeremy spent many hours
with me in the laboratory to ensure I achieved the best results. I also appreciate the immense
contribution of Ray (a former cell culture laboratory technician) during my cell culture assay
in his laboratory. I would also like to thank Eyad for providing all the necessary support and
help for my apoptosis detection assay. I am also grateful to the laboratory technicians in the
Cockroft Building for their unfliching technical and moral support throughout my laboratory
work.
I appreciate all the contributions of my colleagues, the masters and the placement
students in Dave’s laboratory. I would also like to thank Drs James Wilkinson, Elder
Rhoderik and Natalie Ferry for their help and support over the past four years. Jon Deakon is
also highly appreciated for his professional support and help each time I became stuck with
GAGs palava. ELS staff (Catriona and others) have been wonderful and supportive
throughout my study. I also appreciate my mum for coming all the way from Nigeria to help
care for my babies while I was busy writting this thesis. All my friends and family have been
very supportive over the past four years. My sincere thanks also goes to my able boss and
mentors back home, Professors E.O Agbedana, J.I Anetor, J.O Moody, J. Omotade, A.
Sowumi, F.A.A Adeniyi, G.O Arinola and C.O Falade.
xxv
Finally, my sincere appreciation goes to my supervisor, Dr David Pye, for giving me
unrestricted access to his office and providing invaluable advice and support. Without him,
this work could not have been achieved.
xxvi
Abstract
Glycosaminoglycans (GAGs) are a family of complex mixture of linear
polysaccharides that are present in both vertebrates and invertebrates. This polysaccharide
plays important roles in physiological and pathological conditions, including cancer. In this
study, GAGs were isolated from two different fish (whelks and cockles) belonging to mollusc
invertebrates. The crude GAGs isolated from each shellfish demonstrated variable selective
anti-cancer activities against many cancer cell lines including breast (MDANQ01 and
MDA468), leukemia (MOLT-4 and K562) and ovarian (HeLa) cancer. None of the
commercial GAGs exhibited any anti-cancer activities against all the cancer cells studied.
Previous studies conducted on the isolation of GAGs from molluscs reported mainly its anti-
coagulant and anti-inflammatory activities; thus neglecting its record of anti-cancer activity.
All purified whelk fractions (A – D & F) obtained failed to show any anti-cancer
activity; with the exception of fraction E, which showed equal levels of selective anti-cancer
activity against breast cancer cells. Mechanism of cell death caused by the three novel GAGs
on cancers cells were investigated via cell cycle analysis and apoptosis detection assay. Cell
cycle analysis revealed significant perturbations in the cancer cell cycle showing cell cycle
arrests at different stages. Similarly, there were significant apoptosis inductions induced by
the three novel GAGs on each of the cell lines investigated.
Structural elucidations of the two fish GAGs, using chemical, enzymatic,
Polyacrylamide, Superose 12 size exclusion chromatography , gel filtration and SAX-HPLC
methods of analysis, revealed the presence of both chondroitin sulfate (CS)/dermatan sulfate
(DS)-like and HS-like GAGs. Discrepancies in the structural elucidations of the novel GAG
mixtures and the commercial GAGs may be partly responsible for the anti-cancer activity of
the novel polysaccharides, as changes in exogenous GAGs structural composition, especially
sulfation levels or patterns, can alter its binding to growth factors, which is essential for cell
proliferation.
1
Section 1
Introduction and overall aim of this study
2
1.0 General introduction
Glycosaminoglycans (GAGs) are a family of linear, complex, polydisperse
polysaccharides extracted and purified from different animal tissues (Cassaro and Dietrich,
1977; Heinegard and Sommarin, 1987; Pejler et al, 1987a). They are very heterogeneous
polysaccharides in terms of relative molecular mass, charge density, physico-chemical
properties, biological and pharmacological activities (Jackson et al, 1991). GAGs are
ubiquitous in nature, occurring in a wide variety of organisms, including both vertebrates and
invertebrates. They are linked typically to a protein core in order to form proteoglycans.
These anionic polysacharides elicit many biological functions, largely through their
interaction with proteins (Cesaretti et al, 2004). Major GAGs in vertebrates and invertebrates
include heparin, heparan sulfate (HS), chondroitin sulfate/dermatan sulfate (CS/DS), acharan
sulfate (AS), and hyaluronic acid (HA) and keratin sulfate (KS).
All GAGs chains except KS comprise alternating units of an amino sugar, either N-
acetyl-D-glucosamine (GlcNAc) or N-acetyl-D-galactosamine (GalNAc) and a hexuronic
acid (HexA), either glucuronic acid (GlcA) or iduronic acid (IdoA). Keratan sulfate contains
GAGs chains comprising of galactose attached to acetyl-D-glucosamine (Afratis et al., 2012:
Yamada et al, 2011). HS and heparin are the most widely studied of these polysaccharides
due to their involvement in many important biological processes. They have been shown to
play important roles in the control of stem cell growth and differentiation (Patel et al, 2014
and Desai 2013). Moreover, they are involved in a number of important biological activities,
such as developmental processes, angiogenesis, blood coagulation, cell adhesion and tumour
metastasis (Sasisekharan et al, 2006: Wei et al, 2005: Vives et al, 1999: Lindahl et al, 1998:
Salmivirta et al, 1996).
3
HS is also vital in regulation of embryonic development, as well as in
pathophysiological conditions, such as inflammation, wound healing, angiogenesis and
cancer (Tamm et al 2012: Lo et al, 2011: Sasisekharan et al, 2006). These activities are
facilitated by the ability of HS proteoglycans (HSPG) to interact and regulate proteins, such
as enzymes, cytokines, growth factors, and extracellular matrix (ECM) bimolecules (Wei et
al, 2005: Vives et al, 1999). The divergent structure of HS allows it to bind to and regulate
the activity of various growth factors, like fibroblast growth factors 1, 2, 4 etc (FGF-1, FGF-
2, FGF-4 etc), chemokines, morphogens and enzymes at the cell surface and in the ECM:
hence influencing cell adhesion, motility, growth and differentiation (Lo et al, 2011:
Sasisekharan et al, 2006: Vives et al, 1999). The ability of HS to modulate the activities of
many so-called heparin-binding growth factors, serve to co-ordinate the interaction of FGF
with their tyrosine kinase receptors (FGFRs); moreover, this appears to play a critical role in
receptor dimerization and activation (Iozzo and San Antonio 2001: Dickson et al 2000: Vives
et al, 1999: Ernst et al, 1995). The modulatory effect of HS is critical to angiogenesis that
occurs in pathological conditions, including tumour growth and progression; this has been
implicated in the vascularisation of all solid tumours (Iozzo and San Antonio, 2001).
Biological activities of HS depend broadly on the interaction between polysaccharides
and proteins, which appears to be mediated by distinct saccharides sequences within HS
chains. Moreover, the expression of different sequences within the HS chains demonstrates
various levels of specificity, selectivity and molecular organisation. Modulation of tumour
growth occurs through the interaction with angiogenic growth factors, like FGF-10, or with
negative regulators of angiogenesis like anti-angiogenic antithrombin III (Iozzo and San
Antonio, 2001: Ernst et al, 1995).
The modulatory effects of HS on the growth factors and chemokines involved in tumour
angiogenesis have been suggested to be mediated through one of the following mechanisms:
4
The voluntary binding of the growth factors to soluble ECM associated or cell-surface
HS results in the fine control of the bioavailability of growth factors; for example, binding of
tumour growth-factor beta (TGF-β) to betaglycan, a cell-associated PG, and decorin, which is
present in the ECM, and also for fibroblast growth-factor-2 (FGF-2) that binds basement
membrane perlecan in addition to cell-membrane syndecans (Mellor et al, 2007 and
Massague 1992).
The binding of HS to growth factors protects them from proteolytic degradation and
acid inactivation (Samuel et al, 2000: Szabo 1991 and Saksela et al, 1988).
HS modulates the access of FGF growth factors to specific signaling receptors by
different mechanisms that may involve independent interaction of HS with an aspect of the
transmembrane tyrosine kinase glycoprotein component of the FGFR complex (Kan et al,
1993).
HS may also trigger an intracellular transduction signal by interacting directly with
growth-factor receptors with no growth factors being present (Rusnati et al, 1993).
Indeed, Rusnati and others have reported that heparin/HS can activate FGFRs in the absence
of the growth-factor. This observation goes against the traditionally accepted proposal of a
ternary complex involving GAGs, growth factors, and tyrosine kinase (TK) receptors
(Rusnati et al, 1993). The introduction of this model led to an extensive study involving many
research groups and there is still much debate on actual mechanisms by which GAGs mediate
the activation of the FGF’s. Regardless of this debate some general properties of the
signalling complex can be surmised and these are outlined below:
Heparin/HS-related molecules can be useful tools to modulate the biological activity
of heparin-binding angiogenic growth factors and cognate TK receptors (Mellor et al, 2007).
5
Heparin/HS-related molecules can be designed with various structures that are able to
affect differently the biological activities of angiogenic growth (Mellor et al, 2007).
The ideas expressed above show some promise, therefore, there is need for the development
of inhibitors of the activation of growth factors by GAGs and the subsequent development of
new anti-cancer treatments aimed at the inhibition of tumour-cell proliferation.
The ability of low molecular weight heparin fragments administered systemically to
reduce the angiogenic activity of FGF2 and vascular endothelial growth-factor (VEGF)
validate this hypothesis (Ghandi and Mancera, 2010; Norrby 2000: Norrby and Ostergaard
1997 and 1996). Consequently, many HS/heparin fragments and mimics have been shown to
have potential as inhibitors of tumour angiogenesis. In addition to the role played by HS in
regulation of tumour angiogenesis, we shouldn’t forget the potential roles for HS in directly
regulating the growth of cancers through interactions at the tumour cell surface. The
structural complexity of tumour-cell HS (both at the cell surface and extruded into the ECM)
has been shown to play vital roles in tumour development. It enables them to modulate
directly several aspects of tumour-cell phenotype, including growth kinetics, invasiveness
and metastatic potential (Sasisekharan et al, 2002). Hence, a given tumour-derived HS-GAG
or HSPG can be protumorigenic or antitumorigenic, depending on whether it is anchored at
the cell surface or present in the ECM as soluble-free GAGs or/and depending on the HS-
GAG sequence ( Gomes et al., 2013: Liu et al, 2002 and Sasisekharan et al, 2002).
Targeting tumour angiogenesis by interfering with the interaction of HS with
angiogenic growth factors is a well-established model for the development of HS mimetic
therapeutics. However, we shouldn’t forget the ability of HS to modulate the growth and
development of tumours via other mechanisms. This could certainly lead to the determination
of, as yet unknown, HS structures and interactions that could pave way toward the
development of novel cancer therapeutics.
6
The study describe in this thesis employs GAGs derived from shellfish in a novel
approach that targets directly the growth of cancer cells, rather than the vasculature and
angiogenic processes within the tumour. The anti-cancer activity of these shellfish-derived
GAGs is a unique finding, with none of the commercially derived GAGs from mammalian
sources demonstrating any anticancer activity.
The GAGs derived from these shellfish have not been characterised in terms of their
structure, and their therapeutic effect on cancer cells is not reported in the literature.
7
1.1 Glycosaminoglycans
GAG’s are natural heteropolysaccharides, belonging to the family of polyanionic
polysaccharides. These highly negatively-charged polysaccharides are ubiquitous in nature,
occurring in a wide variety of organisms and tissues attached typically to a protein core to
form molecules known as proteoglycans (PGs). They are composed of repeating
disaccharides units comprising either sulfated or non-sulfated disaccharides. Their properties
have been shown to vary considerably depending on the tissue or cell type from which they
are extracted. (Andrade et al, 2013: Vijayabaskar and Somasundaram 2012: Afratis et al,
2011: Heinegard and Sommarin 1987; Pejler et al, 1987: Cassaro and Dietrich 1977).
GAGs elicit numerous biological functions, largely through their interaction with proteins,
including growth factors.
GAGs are found located within the cell mebrane and in the extra-cellular matrix
(ECM). They act by binding selectively to a variety of proteins and pathogens and are crucial
to many disease processes, such as inflammation, neurodegeneration, angiogenesis,
cardiovascular disorders, cancer and infectious diseases (Ghandi and Mancera et al, 2010:
Mark et al 2002).
The GAG family has several archetypal members including heparan sulfate (HS), heparin,
chondroitin sulfate/ dermatan sulfate CS/DS, keratan sulfate (KS) and acharan sulfate (AS).
There is also the non-sulfated GAGs consists of hyaluronic acid HA (Figure 1.1). HA lack a
covalently protein core and are generally synthesised at the intracellular surface of the plasma
membrane. HA GAGs has been reported to be a key player in tissue homeostasis, cancer
progression, inflammatory conditions, myocardial infarction and angiogenesis (Afratis et al.,
2012: Slevin et al., 2002). HS and heparin are the most widely studied members of the
GAG’s family, because of their involvement in many biological activities including
8
angiogenesis, cell proliferation, wound healing, inflammation etc (Afratis et al., 2012: Vives
et al, 1999: Gallagher et al, 1986).
9
Fig. 1.1: Schematic structures of GAGs.
Heparin/HS and HA are glycosaminoglycans; chondroitin sulfate (CS) and dermatan sulfate (DS) are
galactosaminoglycans; KS is a sulfated polylactosamine. Abbreviation: R= H or SO3: R’= SO3 or COCH3
NHCOCH3 OH
COO-
Heparan sulfate
10
1.2 GAG’s structure and functions
GAGs comprise a linear chain of 10–200 disaccharide units of repeating N-acetyl-D-
glucosamine/galactosamine, which is linked to uronic acid (iduronic or glucuronic acid)
(Tumova et al, 2000: Lindahl et al, 1998). The disaccharide repeat unit can be modified to
include N- and O-sulfation and also epimerisation of β-D-glucuronic acid to α-L-iduronic
acid (Conrad, 1998). In addition, the five different modifications for disaccharides give rise to
25 = 32 combinations. Thus, this modification makes the complexity of the GAG much
greater than that of proteins, which are made up of 20 amino acids. With these 32 building
blocks, a GAG octasaccharide could have in excess of a million possible sequences; thereby
making HS-GAGs not only the most acidic, but also the most information-dense biopolymers
found in nature (Conrad, 1998).
The physical form of GAGs and the specific interactions between them and other
ECM components are controlled frequently by the sequence of disaccharide residues that they
are comprised of. Usually, GAGs interact with transient components of the ECM, either at
the cell surface, in solution or sequestered in the matrix. For instance, FGF-2 induced
endothelial-cell proliferation requires trimolecular interactions between FGF-2, FGF -TK
receptors (FGFR) and HS (Jaye et al., 1992: Kiefer et al, 1991: Klagsbrun and Baird, 1991:
Yayon et al, 1991). This interaction activates TK activity of the intracellular domain of the
FGF receptor, which, in turn, leads to secondary messenger activation (Dickson et al., 2000).
11
1.3 Heparin/HS structures and functions
Heparin/HS, usually isolated from animal tissue including vertebrates and
invertebrates, is an important and chemically-distinct polysaccharide of considerable
biological relevance. As explained above they are polydisperse, highly sulfated, linear
polysaccharides, consisting of a repeat unit of uronic acid in either of its glucuronic or
iduronic form attached to D-glucosamine residues (Figure 1.1) ( Koo et al., 2008: Volpi et al,
2005: Islam and Linhardt, 2003). This group of GAGs have a very complex structure yet they
are the most widely studied members of the GAG family. The structural complexity of
Heparin/HS can be considered at both PG and GAG levels;
At the PG level, different numbers of polysaccharide chain (possibly with different
disaccharide sequences) can be attached to the various serine residues present in the protein
core (Koo et al, 2008).
At the GAG level, some of HS/Heparin structural complexity results from their
polydispersity.
GAG especially heparin has a molecular weight ranging from 5-40kDa (degree of
polymerisation (dp) 10-80) with an average molecular weight of 13 kDa. Heparin/ HS
structure has been partially characterised by studying their biosynthesis (Kjellen et al, 1992).
Twelve sulfation profiles for HS/heparin disaccharides have been reported and these have
equally been resolved and characterised by various separation techniques including chemical,
enzymatic, and spectroscopic techniques (Malavaki et al., 2011: Sasisekharan et al., 2006:
Linhardt, 1991).
Problems arise in the structural analysis of HS/Heparin GAGs since they are extensivley
modified by O- and N-sulfation in addition to isomerisation of the iduronic acid making them
12
the most structurally diverse members of the glycosaminoglycan family. The amino group
may be either sulfated or acetylated and each disaccharide unit may have up to three of the
hydroxyl groups sulfated (2-O-S, 3-O-S and 6-O-S). Glucuronic acid rich polymers are
sometimes classed as HS while the iduronic acid rich polymers are also sometimes refers to
as heparin. Heparin contain a pentasaccharide region (GlcNAc/NS(6S)-GlcA-GlcNS(3S,6S)-
IdoA(2S)-GlcNS(6S) that bind to antithrombin III and this makes it the most widely used
carbohydrate based therapeutic because the binding allows it to inhibit blood coagulation
(Loganathan et al,1990: Marcum and Rosenberg,1989a: Linhardt et al,1988b: Atha et
al,1985: Lindahl et al, 1984). Relating structure to biological activities, such as that described
for heparin, is critical in our understanding of the role sulfation patterns and epimerisation
play in the natural function of heparin/HS chains.
Sulfation patterns of HS/heparin play a very crucial role in their interactions with growth
factors, proteins and cytokines, and therefore may affect their biological roles. HS/heparin
have been implicated in numerous biological processes at the cell–tissue–organ interface (
Malavaki et al., 2011: Conrad 1998), which are triggered mainly by their interactions with a
wide range of proteins, such as cofactors of the coagulation cascade, extracellular-matrix
components and a variety of cytokines and growth factors (Vives et al 1999: Permimom and
Belfield, 2000), angiogenesis (Sasisekharan and Venkataraman, 2000), viral invasion (Shukla
et al, 1999 and Chen et al, 1997), and anticoagulation (Petitou et al, 1999).
The HS/heparin also exerts its modulatory effects on key biological processes by binding
to growth factors, cytokines, morphogens, enzymes and other signaling molecules (Taipale
and Keski-Oja, 1997). They can regulate the activity of signaling molecules by modulating
their diffusion, receptor on and off rates, and effective concentration at the cell surface and
13
the ECM, However, these processes become especially important at the cell–tissue–organ
interface.
Previous studies have added an extra dimension to this cell-surface event by indicating
that HS mediates dimerization, either of FGF-2 of FGF receptor or of both, which may be a
requirement for signal transduction (Ornitz et al, 1996: Pantoliano et al, 1994: Springer et al,
1994: Mascarelli et al, 1993: Ornitz et al,1992). The binding of HS chains to FGF-2 and
FGFR occurs through N- sulfated glucosamine (GlcNS) and 2-O-sulfated iduronic acid
(Ido2S) units or 6-O- sulfated glucosamine (Glc6S). Once the FGFs bind to their receptors,
FGFR complexes dimerise, in conjuction with HS/heparin moiety, leading to the activation of
tyrosine kinase through autophosphorylation. Ultimately, these events facilitate the binding of
second messenger proteins which in turn trigger many other intracellular signalling
(Gallagher 2001: Dickson et al 2000).
The various roles played by these polysaccharides are becoming clearer as researchers
continue studying them.
1.4 CS structure and functions
Chondroitin and dermatan sulfate make up a second GAG family, also known as
galactosaminoglycans. These polysaccharide chains are, again as in HSPG’s, normally found
covalently bound to a protein core forming high molecular weight units, with a large number
of GAG chains attached (Ernst et al, 1995). The basic structural unit of this class of GAG is a
disaccharide in which a uronic acid (D-glucuronic and L-iduronic acid) is attached (β1→3) to
N-acetyl galactosamine (Figure 1.1). CS is the most abundant GAG in the body skeletal
muscle and soft tissue.
14
There are various sulfation patterns of CS and among the most studied sulfated CS
GAGs are the two common isomers CS-A (O-sulfo group attached at position 4 of galactosyl
residue) and CS-C (O-sulfo group attached at position 6 of galactosyl residue) see Figure 1.2.
Similarly, disulfated CS are also classified as CS-D (O- sulfo group attached at position 2 of
glucuronic acid and position 6 of galactosyl residue) or CS-E (O- sulfo group attached at
position 4 and 6 of galactosyl residue). The other CS isoform formerly designsted as CS-B is
called DS which is characterised by the presence of IdoA moiety in his disaccharide chains.
Similar to HS/heparin, the various sulfation patterns of CS GAGs enable specific interaction
with many molecules, including growth factors, cytokines, chemokines, adhesion molecules
and lipoproteins (Asimakopoulou et al., 2008).
The size of CS chains varies greatly, with an average of about 40 repeating
disaccharides units for the cartilage proteoglycans, corresponding to a molecular weight of
approximately 20,000 (Iozzo, 1985). Their sulfo group content also varies depending on the
number(s) attached to both or either of the galactosyl and uronic acid residues (Iozzo, 1985).
Once again they all show a considerable degree of microheterogeneity within the polymer
chain in a manner very similar to HS. The disaccharide unit present in CS/DS may be non-
sulfated, mono-sulfated or disulfated and both iduronic and glucuronic acids may be present
in a given polymer chain.
DS (CS-B) is a polydisperse; microheterogenous sulfated copolymer of D-Gal-NAc
and primarily L- iduronic acid (L-IdoA), with O-Sulfate groups most commonly attached to
position 4 of the galactosyl residue and position 2 of the L- Iduronic acid residues (Linhardt
and Hileman, 1995). Many DS core proteins such as decorin and biglycan have been
identified (Kresse et al, 1993: Coster, 1991). Decorin and biglycans have been reported to
play vital roles in many biological activities including organisation of collagen fibrils,
15
regulation of the extravascular activities of thrombin, act as anticoagulants by inhibiting
thrombin and lipid metabolism (Pangrazzi and Gianese, 1987). ). CS-B or DS is abundant in
skin and is also found in heart valves, tendons and arterial walls. It is made up of linear
repeating units containing D-galactosamine and either L-iduronic acid. Its molecular weight
ranges from 15,000 to 40,000 daltons.
Moreover, CS-A is commonly found in humans in cartilage, bone, cornea, skin and
the arterial wall. The molecular weight of CS-A ranges from 5,000 to 50,000 daltons and
contains about 15 to 150 basic units of D-galactosamine and D-glucuronic acid (Wastenson,
197). CS-C, is primarily found in fish and shark cartilage, but also in humans, is also made
up of linear repeating units of D-galactosamine and D-glucuronic acid.
16
Figure 1.2: Structure of different types of CS
(A) Chondroitin-6-Sulfate; (B) DS; (C) Chondroitin-4-Sulfate
Chondroitin A B C GAGs
17
1.5 Glycosaminoglycans isolated from shellfish
Many researchers, including Dietrich and co-workers, reported the isolation of GAGs
similar to heparin with comparable anti-thrombin activities from mollusc’s invertebrates.
Similarly, heparin-like substance with relative ability to bind antithrombin III (ATIII) has
been isolated from the marine clams, anomalocardia brasiliana (Pejler et al, 1987: Dietrich et
al, 1985). Another GAG similar to heparin GAG, with an AT-binding region comparable to
that of mammalian heparin has also been purified from another clam species, Mercenaria
mercenaria (Jordan and Marcum, 1986). Additionally, heparin, (a highly sulfated
polysaccharide, commonly isolated from mast cell or mucosa and also used as an
anticoagulant in the clinic) (Bjork and Lindahl, 1982) has been reported to have some other
biological activities, such as; anti-viral activity, bind to a variety of growth factors, inhibit
complement activation, and regulate angiogenic activity (Weiler et al, 1992; Jackson et al,
1991; Casu 1985; Folkman et al, 1983).
1.6 Biosynthesis of GAGs
HS and CS are synthesised in the Golgi, whereby the individual GAG chains are O-
linked to a core protein, forming a large polysaccharide-protein conjugate known as
proteoglycan (PG) (Sasisekharan et al, 2006: Silbert and Sugumaran, 2002: Sugahara and
Kitagawa, 2002). However, KS can be either N-linked or O-linked to the core protein of the
PG (Funderburgh 2002). HA is not synthesised in the Golgi from the core protein but rather
by an integral plasma membrane synthase, which secretes the nascent chain immediately
(Itano and Kimata, 2002). All GAGs, with the exception of HA, are biosynthesised as
proteoglycans and the linkage region is the same in all, except for keratan sulfate. This
18
linkage region consists of the tetrasaccharide; glucuronic acid (GlcA), galactose (Gal), Gal,
and xylose (Xyl)-linked to the hydroxyl group of serine in the polypeptide core (Sugahara
and Kitagawa, 2000). Biosynthesis of all GAGs, except HA is initiated from a core protein,
rich in serine-glycine repeats, which create the platform for the attachment of one or more
GAG chains via the linkage region (Kimura et al, 1984). Contrarily, HA GAGs lack a
covalently bound protein core and is synthesised at the intracellular surface of the plasma
membrane (Afratis et al., 2012)
Biosynthesis of GAG is a complex non-template-driven process that involves many
enzymes that assemble the GAG polymer and then sulfate them at specific positions. GAGs
are synthesised as homopolymers, which are modified subsequently by N-deacetylation and
N-sulfation. This is followed by numerous modifications, including sulfation, epimerisation
and desulfation; all of which are performed in a spatiotemporal manner, producing mature
and functional GAG chains that exert biological functions dependent on their specific
structure. This is common to both types of GAG chain and is formed through the stepwise
addition of each monosaccharide residue by the respective specific glycosyltransferase
(Grimshaw,1997).
After the attachment of the linker, the first modification to the chain determines
whether the chain matures into a CS or HS. This modification involves the transfer of a
GlcNAc (HS) or a GalNAc (CS) monosaccharide. The enzyme GlcNAcT-I transfers GlcNAc
to the tetrasaccharide linker, initiating HS biosynthesis (Rohrmann et al, 1985). This enzyme
is different from the glycosyltransferase GlcNAcT-II that is involved in the elongation of the
HS GAG chains. In the case of CS, the initiating GalNAc residue is transferred to the linker
region by the enzyme GalNAcT. It is not very clear whether the activity of this enzyme
differs from the GalNAc transferase activity of chondroitin synthase, which is involved in the
19
chain-elongation process. In all cases real chain-building ensues after the transfer of GlcNAc
(HS) or GalNAc (CS) to the linker.
In the case of HS chains, a multidomain glycosyl-transferase successively adds
GlcNAc and GlcA; thus, initiating the chain-elongation process. This multidomain enzyme is
encoded by EXT1 and EXT2 of the EXT family of genes. Although EXT1 and EXT2 possess
the ability to transfer both GlcNAc and GlcA, it has been established that these enzymes form
a single oligomeric unit, which is required for complete in vivo chain-elongation activity.
Similarly, in the case of CS, chondroitin synthase, also a known multidomain enzyme,
transfers GalNAc and GlcA successively for chain elongation (Sashisekhare et al, 2006).
Molecular cloning has been achieved for four of the glycosyl transferases responsible for the
biosynthesis of the linkage region tetrasaccharide (Uyama et al, 2007: Kitagawa et al, 1998).
Firstly, xylosyl transferase (XylT) transfers a Xyl residue from UDP-Xyl to specific
serine residues in core proteins in the endoplasmic reticulum and the cis-Golgi compartments
(Figure 1. 3) (Uyama et al, 2007). Secondly, Two XylTs, XylT-1 and XylT-2, were cloned,
and their amino acid sequences found to be significantly homologous. In contrast enzymatic
activities were only shown by XylT-1, not by XylT-2. Following the transfer of a Xyl
residue, two Gal residues are transferred to the Xyl residue by two kinds of galactosyl
transferases (GalTs), GalT-I and GalT-II, in the cis- 1-O-Ser, in the medial- and trans-Golgi
compartments (Figure 1.3) (Uyama et al, 2007).
20
Figure 1.3; Schema of the biosynthetic assembly of the GAG backbones by various
glycosyltransferases.
A number of glycosyltransferases are required for the synthesis of the backbones of GAG’s.e.g XylT, Xyl
transferase; GalT-I, Gal transferase-I; GalT-II, Gal transferase-II, GlcAT-I, GlcA transferase-I; GalNAcT-I,
GalNAc transferase-I; CS GlcAT-II, CS GlcA transferase-II;GalNAcT-II, GalNAc transferase-II; CS
polymerase, GlcA/GalNAc transferase; GlcNAcT-I, GlcNAc transferase-I; GlcNAcT-II,GlcNAc transferase-II;
HS polymerase, GlcA/GlcNAc transferase; ChSy-1, chondroitin synthase-1; ChSy-2, chondroitin synthase-2;
and ChPF, chondroitin polymerising factor.
The biosynthesis of the linkage region is completed by the actions of GlcAT-I;
transferring a GlcA residue to the linkage trisaccharide, Galβ1→3Galβ1→4Xylβ. Moreover,
one study highlights that the expression level of GlcAT-I correlates well with the amount of
Heparan sulfate/Heparin
Chondroitin sulfate/Dermatan sulfate
21
GAGs; thereby suggesting that GlcAT-I regulates the overall expression of GAGs (Uyama et
al, 2007). The resulting GAG chain backbone undergoes extensive sulfation modifications,
during chain elongation, thus making GAG chains some of the most negatively-charged
families of biopolymers in mammalian cells.
1.7 Biosynthetic modification of HS-GAG chain (HS chain elongation)
The nascent HS chain is first modified by N-deacetylase, N-sulfotransferase (NDST),
which is a multidomain enzyme that cleaves the N-acetyl group from the GlcNAc
monosaccharides and transfers a sulfate group to the N-position. This is followed by the
action of the C-5 uronyl epimerase, which converts GlcA to IdoA (Figure 1.4) in selected
positions. 2-O-sulfation of the uronic acid by the 2-O sulfotransferase (2-OST) can follow the
epimerisation process. The 2-OST acts on IdoA- as well as GlcA-containing HS chains;
however, the IdoA containing chains are the catalytically preferred substrates (Pinhal et al,
2001: Rong et al, 2001). The final set of modification enzymes are the 6-O (6-OST) and 3-O
(3-OST) sulfotransferases, which sulfate the 6-O and 3-O positions of the GlcNAc moiety,
respectively. Many of the above biosynthetic enzymes have distinct isoforms that are
selectively expressed in different tissues (Kusche-Gullberg and Kjellen 2003). Four different
isoforms of NDST, three different 6-OSTs, and six different 3-OSTs have been characterised
in humans and mice (Kusche-Gullberg and Kjellen 2003), they all have different specificities
and as a result the wide diversity of HS chains produced by animal cells.
22
Figure 1.4 HS chain elongation
The chains are synthesised on the core protein by the sequential action of individual glycosyl transferases. A
common tetrasaccharide linkage region is formed, followed by the addition of alternating GlcA and GlcNAc
residues, producing in turn the precursor chain. This chain is then enzymatically modified by deacetylation and
N-sulfation, epimerisation and O-sulfation, yielding individual chains whose sequence is distinct from all the
other chains.
GLCNAc/GlcA
transferase
(tout velu/Ext)
UDPglucose
Dehydrogenase
sugarless
N-deacetlase/
N-sulfotransferase
(sulfteless)
GlcA C5-epimerase
2,6-and 3-O-
sulfotransferase
UDP-
GlcNac
UDP-GlcA
GlcA
IdoA
PAPS
Sulfate
Core protein
Linkage region
23
1.8 Biosynthetic modifications of CS/DS GAG chains (CS/DS chin elongation)
CS/DS sulfated GAGs [(CS] are covalently attached to their respective core proteins
through the GAG–protein linkage region, GlcAβ1→3Galβ1→3Galβ1→4Xylβ1→O-Ser
(Figure 1.3). The biosynthesis of CS can be broadly divided into that of chondroitin and DS.
CS is comprised of predominantly the GlcA epimer, whereas dermatan is predominantly
comprised of IdoA. Thus, the CS C-5 uronyl epimerase is more prominent in the biosynthesis
of DS. The first GalNAc transfer to the linkage region by the alleged GalNAc transferase-I
leads to the synthesis of the repeating disaccharide region [(→4GlcAβ1→3GalNAcβ1-)n] of
CS/DS through alternate additions of β-GalNAc and β-GlcA by the concerted actions of the
putative GalNAc transferase-II and GlcA transferase-II enzymes, which are specific to CS
backbone synthesis (Figure 1.5).
The three main sulfation events of the CS chains are 4-O and/or 6-O-sulfation of
GalNAc and 2-O-sulfation of uronic acid. There are four different isoforms of the CS
GalNAc 4-OST (C4ST-1, C4ST-2, C4ST-3, and D4ST-1) and three different isoforms of the
CS GalNAc 6-OST (C6ST, C6ST-2, and GalNAc4S-6ST) (Kusche-Gullberg and Kjellen
2003).
24
Figure 1.5; Pathways of CS/DS chain elongation.
C4ST, chondroitin 4- O -sulfotransferase; C6ST, chondroitin 6- O -sulfotransferase; D4ST, dermatan 4- O -
sulfotransferase; CS/DS2ST, uronyl 2- O -sulfotransferase; Gal-NAc4S-6ST, GalNAc 4-sulphate 6- O -
sulfotransferase; O unit, GlcA b 1-3GalNAc; iO unit, IdoA a 1-3GalNAc; A unit, GlcA b 1-3GalNAc(4S); iA
unit, IdoA a 1-3GalNAc(4S); iB unit, IdoA(2S) a 1-3GalNAc(4S); C unit, GlcA b 1-3GalNAc(6S); D unit,
GlcA(2S) b 1-3GalNAc(6S); and E unit, GlcA b 1-3GalNAc(4S,6S).
25
1.9 Analysis of GAGs and their oligosaccharide fragments
There are various ways to study the biological function of GAGs structures in order to
understand the structure-activity relationships (SAR). Traditionally, the determinations of
GAG’s structures are usually derived from the following steps:
Direct extraction and purification of HS populations from tissues or culture cells arising
from different organs.
Partial chemical and enzymatic modifications of GAGs to produce oligosaccharides of
defined modifications and size (Yates et al, 2004). The structure of these fragments can
be confirmed using disaccharide compositional analysis as well as sequencing methods.
Chemically synthesised GAGs oligosaccharides (Grootenhuis et al, 1995) may shed light
on specific HS structure activity relationships. Synthesis of GAGs structures is a very
long and specialized process. However, solid-phase synthesis and combinatorial
chemistry has greatly advanced this field in recent years (Vohra et al, 2008: Seeberger
and Werz, 2005: Seeberger and Haaze, 2000)
1.10 Traditional methods for extraction and purification of GAGs from Tissue
Samples and Cultured Cells
In general, extraction of GAGs is initiated by the action of proteolytic enzyme
(e.g.Alcalase) on the core protein of PGs. This enzyme degrades the core protein into short
peptides, thereby releasing the corresponding GAGs chain. Dialysis with high concentrations
of harsh organic solvents such as 8 M urea and addition of trichloroacetic acid (Lyon and
Gallagher, 1991) or guandinium chloride are also employed (Yanagishita et al, 1987). These
chemicals are chaotrophic agents that are capable of disrupting the three-dimensional (3D)
26
structures of proteins, DNA and RNA. Urea and other chaotrophic agents usually disrupt the
3D structure of proteins by interfering with the stabilizing inter-molecular interactions which
mediate non-covalent forces such as hydrogen bonds, van der Waals forces and hydrophobic
effects (Puvirajesinghe and Turnbull, 2012). The disadvantages of these methods include:
they are lengthy; they can involve multiple sample transfers; they can contain harsh
chemicals; and they may alter pH and cause de-N-sulfation (Inoue and Nagasawa, 1976).
Other methods include β-elimination, which involves alkaline borohydride treatment, which
also acts to disrupt the serine-xyloside linkage that attaches GAG chains to the core protein
backbone; all these methods result in the release of intact GAGs from protein cores (Stenstad
et al, 1993).
Another method that can be used for GAGs purification, from cultured cells, involves
the use of a non-ionic detergent solution, such as 1% Triton X-100 0.5 M KCl, which can
then be subjected to density centrifugation using caesium chloride gradients. This separates
the molecules according to their density (Jalkanen et al, 1988). Electrophoretic techniques
can be used for separation of proteoglycans. This technique can be used either separately or
in combination with SAX-chromatography, depending on the degree of purification required
or type of HSPG to be purified.
1.11 Chemical and enzymatic depolymerisation of GAGs used in structural analysis
The polydisperse nature and large size of GAG chains means that it impossible to
determine the structure of individual GAG chains. Structure activity relationships between
GAG chains and proteins must therefore be determined by reducing the size of the chains into
more manageable oligosaccharides. The most common method of determining differences in
27
GAGs derived from a variety of sources is the analysis of disaccharides composition, which
is commonly achieved by depolymerisation of the GAGs chain by chemical or enzymatic
treatment. Site-specific enzymes are used to degrade the polysaccharides for structural and
analytical purposes (Murata and Yokoyama, 1987: Linhardt 1986). Depolymerisation of the
polysaccharides can results in the creation of smaller saccharides chains, known as
oligosaccharides by partial degradation enzymatic or chemical treatment.
They can also be degraded further by a combination of site-specific enzymes in order
to yield disaccharides, subsequent analysis by SAX-HPLC can give the total disaccharide
composition of the GAG chains. While similar disaccharides may be present in different
tissues, the proportion of each varies considerably thereby allowing the identification of
structural differences between tissues. Furthermore, the domain structures of GAGs can be
analysed to understand the relative distributions of nonsulfated and sulfated domains from
different cells and tissues (Esko and Lindhart, 2001). The structures found in different
domains can be analysed further using oligosaccharide mapping, which provides a
‘fingerprint’ of the domain structures (Turnbull and Gallagher, 1991: Turnbull 1990:
Turnbull and Gallagher, 1988). The development of GAG sequencing technology has been
used to provide more detailed information on the structure of individual oligosaccharides
involved in important biological interactions (Turnbull et al, 1999). GAG oligosaccharides
structures have been studied extensively by using one or more of the following methods and
have provided a wealth of information on the relationships between the fine structures of
GAG chains.
Originally, depolymerisation of HS/heparin was achieved using nitrous acid
hydrolysis. Nitrous acid cleaves in between the hexosamine residues and the hexuronate
residues, where the amino group is either N-sulfated or unsubstituted. This result in the
28
conversion of the D-glucosamine at the reducing end of the structure into a 2, 5- anhydro-D-
mannose residue and the hexuronate residues remain intact (Burdon and Van Knippenberg,
1985). This reaction has been studied extensively and is proven to be pH-dependent. Direct
deamination of N-sulfated glucosamine residues is possible at a low pH condition (< 2.5).
However, N-unsubstituted residues are deaminated more rapidly at an optimum pH 4
(Shively and Conrad, 1976).
This method cannot be used to fully characterise the GAG oligosaccharides directly as
the depolymerisation process does not generate a suitable specific chromophore, in other
words, chemical digestion and separation of such fragments can be followed only at low
sensitivity by spectroscopic detection (Powell et al, 2004). Increased detection sensitivity is
achieved by combining nitrous acid degradation with reducing end labelling methods, such as
radiolabelling, or fluorescent tags. The labelling reaction of the reducing end of nitrous acid
treated fragments is aided by the fact that the 2, 5- anhydro-D-mannose residue produced at
the reducing end is highly reactive (Puvirajesinghe and Turnbull, 2012). Furthermore, this
method is limited by its ability to cause reduced yield due to ring contraction of uronic acid
residues or p-elimination of the glucuronic acid (Guo and Conrad, 1989).
1.12 Use of separations techniques for structural analysis
GAGs can be analysed in many different ways, the choice of techniques depending on
factors such as the source and quantity of materials, the type of data required and the
preparation and/or treatment of GAGs prior to the analysis process. NMR spectroscopy and
mass spectrometry are useful techniques for such analysis and have been able to provide
direct sequence information (Kitagawa et al, 1995). However, both techniques require
29
specialized instruments, which are not routinely available and NMR in particular requires
relatively large quantities of materials (millimolar to micromolar quantities). These
drawbacks leave chromatographic techniques as the most common and easiest methods used
to examine GAGs structure (Puvirajesinghe and Turnbull, 2012).
1.13 Strong anion-exchange chromatography (SAX-HPLC)
To date, chromatography remains the most reliable technique for the routine
separation of GAGs and the common ones generally in use are gel chromatography and high-
performance liquid chromatography (HPLC). Oligosaccharide products can be purified and
separated according to their molecular weight and other properties such as charge and
hydrodynamic volume (Puvirajesinghe and Turnbull, 2012). Several methods, such as
radioactivity measurement, UV detection at 232 nm, fluorescence detection, can be used for
detection. Radioactivity measurement can be used to detect 35
S and 3H in samples prepared
by biosynthetic radiolabelling (e.g., cultured cells) or where oligosaccharides (digested using
nitrous acid) are labelled at their reducing-ends with 3H–borohydride and UV detection at
232 nm can also be used to detect the disaccharide products. Another UV wavelength
commonly used is 215 nm, which detects acetyl bonds, although this is less sensitive than
detection at 232 nm. Fluorescence detection is another reliable and extremely sensitive
method that can be used to detect fluorescently-tagged oligosaccharides. Strong anion-
exchange chromatography (SAX-HPLC) techniques are used for the separation of structures
according to their negative charge content. A common column is the Pro-Pac PA1, which is
made of quaternary ammonium functional groups attached to nonporous core particles by
agglomerated MicroBead™ resin. SAX-chromatography can be used in combination with
PAGE separation, for the purification of GAGs oligosaccharides (Vives et al, 2001).
30
1.14 Polyacrylamide Gel Electrophoresis (PAGE)
Electrophoresis is primarily an analytical technique for charged molecules. It is a technique
that separate GAG oligosaccharides based on their mass to charge ratio (m/z). Although,
PAGE analysis is one of the common biochemical techniques used for the separation of
protein and DNA, it has also been used to separate GAG samples in a similar manner for its
use in the analysis of DNA and protein (Wong et al 2006). However, PAGE analysis of GAG
oligosaccharides was initially complicated because of the demand for high resolution due to
the polydispersity and structural heterogeneity of GAG samples: this drawback has now been
resolved by the introduction of discontinuous gel electrophoresis, together with the
development of specialised stacking gels and buffer (Rice et al 1989).
The use of fluorescent tags to label digestion products at their free reducing-ends via
reductive amination reaction has also been determined and this has led to a technique known
as flourophore-assisted carbohydrate electrophoresis (FACE). The enzymes-digested
products can be stoichiometrically coupled to a fluorescent tag and separated using high
percentage gels. Picomolar concentrations can be viewed using a transilluminator
(Puvirajesinghe and Turnbull, 2012).
1.15 GAG’s degrading enzymes
Overall GAG’s degrading enzymes are an extremely important tool in relating GAG
structure/sulfation pattern to biological activities therefore an understanding of the
specificities of these enzymes is crucial to interpreting the data generated by the action of
these enzymes on GAG chains. The most widely used enzymes are a family of structurally
related heparin/HS lyase and their properties and specificities are described below.
31
1.16 Heparinases
Heparinases are enzymes lyases that can eliminatively cleave heparin or HS into
disaccharide and oligosaccharide products: they are also involved in the release of heparin-
bound growth factors from the ECM (Kim et al, 2000). Six different heparinase enzymes
have been isolated from four different bacteria namely: Flavobacterium heparinum, Bacillus
sp., Bacteroides heparinolyticus, and an unclassified soil bacterium (Yoshida et al, 2002). At
least 29 other bacteria expressing heparinase activity as determined by a qualitative plate
assay has been isolated. (Yoshida et al, 2002: Steyn et al,1992: Salyers et al, 1977).
Fractionation of crude heparinase afforded three different heparinases usually called lyases I,
II and III, each of which have a different substrate specificities (Figure 1.6) (Desai, 1993).
The individual heparinase enzymes cleave unique glycosidic linkages, allowing Heparin and
HS to be degraded to specific types of oligosaccharide fragments which vary in length and
sulfation pattern (Linhardt et al, 1990).
Isoelectric focusing (PI) showed that Bacillus species heparinase (PI = 6.6) has an
overall negative charge at its optimal pH of 7.5 while all three F. heparinurn heparinases (PI
= 8.5- 10.1) are positively charged at their pH optima of 7-7.5. For enzymes that degrade a
polyanionic substrate, this appears to be an important difference that may imply different
mechanisms for heparinases from Bacillus sp. and from F. Heparinum (Lohse and Linhardt,
1992). However, the temperature optimum for Bacillus sp. heparinase is 50°C but 90% of the
activity is lost after 3h at 45°C (Bellamy and Horikoshi, 1992). Moreover, for short digest
sodium phosphate buffer has been reported to give higher activity than sulfonate-based
buffers (MOPS, TES, and HEPES), but the latter seem to increase stability of heparinase’s I,
II, and III (Lohse and Linhardt, 1992). It appears in general that the optimal conditions for
heparinases are different depending on the durations of the assay but there is some
32
controversy about this finding which could be critical in determining the completeness of
GAG digestions.
There is very important substrate specificity associated with heparin lyases, which has
been defined as a disaccharide containing a cleavable linkage. Heparinase I cleaves the
linkages HNS (6X)-I-2S [GlcNS (6S) (1 → 4) IdoA2S], heparinase II the linkages HNY,6X- G/I2x
[GlcNS (6S) (1 → 4) IdoA (GlA) 2S], and heparinase III the linkages HNAc-I and HNY,6X-G
[GlcNAc(1 → 4) IdoA] and [GlcNS (6S) 1 → 4) GlcA)], in which H is glucosamine, I is
iduronic acid, G is glucuronic acid,Y is sulfated or acetylated (CH3CO or SO3) and X is
sulfated or unsubstituted (H or S03).
Figure 1.6: Primary glycosidic linkages cleaved by Heparin lyases.
Abbreviations: X, H or SO3−; Y, CH3CO or SO3−. Heparin lyase II cleaves at either glucuronic or iduronic
acid residues.
The enzymatic action of individual heparinases leads to the generation of
oligosaccharides with specific structural features. Degradation of HS with all the three
heparinases reduces HS chains to their disaccharide components, an essential property in
structural characterisation. These disaccharide units comprises of ∆4,5
-uronic acid attached to
N-acetylglucosamine at the reducing terminus and with varying degrees of sulfation (Lohse
33
and Linhardt, 1992). Both D-glucuronic acid and L-iduronic acid give the same ∆4, 5
-uronic
acid after enzyme treatment (Lohse and Linhardt, 1992). The main disaccharides found in
HS/heparin and their traditional abbreviations are; Δ-UA-GlcNAc (IVA); Δ-UA-GlcNS
(IVS); Δ-UA-GlcNAc (6S) (IIA); Δ-UA(2S)-GlcNAc (IIIA); Δ-UA-GlcNS (6S) (IIS); Δ-UA
(2S)-GlcNS (IIIS); Δ-UA(2S)-GlcNAc (6S) (IA);Δ-UA (2S)-GlcNS (6S) (IS).
1.17 Heparinase I from F. heparinum (EC 4.2.2.7)
Heparinase I has also been shown to cleaves heparin at both the GlcNS (6S) (1 → 4) IdoA
(2S) and GlcNS (3S,6S) (1 → 4) IdoA (2S) linkages (Xiao et al 2011). The GlcNS(3S6S) (1
→ 4) IdoA(2S) linkage, found primarily within the antithrombin III binding site, is more
susceptible to heparinase I than the major heparin disaccharide repeating unit GlcNS(6S) (1
→ 4) IdoA(2S). The complete depolymerisation of heparin by heparinase I has been reported
to mainly produce eight different disaccharides (Linhardt et al., 1992).
34
Figure 1.7: Unsaturated disaccharide derived from HS by enzyme catalysed
elimination.
1.18 Heparinase II from f. heparinum
Heparinase II is also active on both heparin and HS, with the HS activity being
approximately twice as high as the heparin activity (Lohse and Linhardt 1992: Linhardt et al,
1990: Nader et al, 1990). The distribution of products for heparinase I1 degradation of
heparin is not as well characterised as for heparinase I and appears to reflect the composition
of the substrate. Heparinase II degradation of heparin yields predominantly the trisulfated
disaccharide structure with other minor detectable disaccharides being produced; this fits
with the highly sulfated nature of the heparin polymers. Moffat and others have reported a
broad substrate specifity of this enzyme. A characteristic that is contrary to the general
property of enzyme reported previously (Desai et al., 1993a: Moffat et al, 1991a).
Furthermore, this enzyme has been demonstrated as capable of cleaving both of the
isomeric forms of uronic acids (IdoA and GlcA) even though the epimerised C5 hydrogen is
being abstracted in the reaction (Desai et al, 1993). This is unusual for enzymatic reactions
which are normally stereospecific due to the defined structure of the enzyme catalytic site.
35
The susceptible linkages are HNY,6X-U2X where the uronic acid can be IdoUA or GlcUA, the
X group can be sulfated or unsubstituted, and Y can be either sulfated or acetylated but not
free.
1.19 Heparinase III from f. Heparinurn (E.C 4.2.2.8)
Heparinase III is less active on standard heparin or heparin-like segments of HS, i.e.
highly sulfated polymers and specifically degrades mono- or non-sulfated sequences within
HS chains. None of the standard methods of oligosaccharides analysis of GAGs such as,
SAX-HPLC (Linhardt et al., 1990), capillary zone electrophoresis (CZE) electropherograms
(Ampofo et al., 1991), gradient PAGE (Desai et al., 1993a) yielded any appreciable
disaccharide degredation products when heparin was incubated with heparinase III. The
degradation products from heparinase III degradation of HS are poorly non- and mono-
sulfated disaccharides, indicating a preference for the enzyme to degrade less modified
regions of the polymer.
Previous studies conducted by Rice and colleagues have also highlighted that
heparinase III is more active towards larger oligosaccharides than the smaller ones. It has also
been shown to be active towards oligosaccharides with N, 6-disulfated (NS6S) or N-
acetylated hexosamine (Linhardt et al, 1990: Rice and Linhardt, 1989). These findings have
resulted in speculation that N-sulfation and 6-O-sulfation do not inhibit cleavage by this
enzyme. This was confirmed by the existence of 6-O-sulfated and N-sulfated products
following cleavage of polymeric HS with heparinase III (Moffat et al, 1991).
36
1.20 Chondroitinases
Chondroitinase enzymes are once again extremely important tools for the structural
characterisation of GAGs and have been isolated and characterised from bacteria of the
genera Arthrobacter, Flavobacterium, Aeromonas, Bacillus, Bacteroides, Proteus and an
unclassified strain possibly Aurebacterium (Earnst et al, 1995: Yamagata et al, 1968).
Chondroitinase-ABC (EC 4. 2. 2. 4) is a general purpose enzyme that cleaves all glycosidic
linkages in the three members of the CS group and also with hyaluronan. It is been classified
as a remarkable enzyme because of its ability to cleave linkages with iduronic acid as well as
linkages with its isomer, glucuronic acid (Linhardt et al 2006).
In addition, chondroitinase activity has been detected in several other microorganisms
(Linhardt et al., 1986: Salyers et al., 1977). It is an extremely important tool used to
completely degrade CS/DS to their disaccharide components, which can be quantified by
SAX-HPLC, CE, FACE, PAGE, etc. It acts on chondroitin 4-sulfate, chondroitin 6 sulfate,
and DS, and acts slowly on hyaluronate (Figure 1.8). Inability of the chondroitinases to show
any activity towards heparin or HS, which are entirely 1 4 linked indicates, that the 1 3
linkage of CS is a requirement for its enzymatic activity (Linhardt et al, 1986: Salyers et al,
1977).
37
Figure 1.8: Glycosidic linkages cleaved by chondroitin lyases.
Abbreviation: Ac, CH3CO.
Chondroitinase-B lyase (EC 4.2.2.19) is specific for DS degradation and the resulting
oligosaccharides as resolved by SAX-HPLC has been reported by Linhardt and others to
yield ΔUA-GalNAc (0S); ΔUA-GalNAc6S (6S); ΔUA-GalNAc4S (4S); ΔUA2S-GalNAc4S
disaccharides accounted for 50 to 65% of the 232 nm absorbance while the remaining 35 to
50% absorbance most likely originated from unidentified oligosaccharides (Linhardt et al,
1991). However, degradation of oversulfated DS GAG chains isomers additionally yielded
the trisulfated disaccharide, ΔUA (2S)-GalNAc (4S, 6S) (Figure 1.9) (Murata and Yokoyama,
1987). Purification of the crude enzyme by column chromatography over hydroxyl apatite led
to discovery of chondroitinase-AC lyase (4.2.2.5) which only eliminates the amino sugar
attached to glucuronic acid and to chondroitinase-B lyase which eliminates amino sugars
attached to iduronic acid (Gu 1995). Separation of the hydrolysis products by SAX-HPLC
Chondroitin ABC lyase Chondroitin ABC lyase
Chondroitin ABC lyase
Chondroitin sulfate E
Oversulfated chondroitin
Chondroitin sulfate D Unsulfated chondroitin Chondroitin sulfate A
Chondroitin ABC, B lyase chondroitin ABC, AC lyase
Chondroitin ABC, AC lyase Chondroitin ABC, AC lyase
Chondroitin sulfate B chondroitin sulfate C
38
after treatment of GAGs with AC/ B lyases provides useful analytical information on their
structure. They are also powerful tools used to generate CS/DS oligosaccharides and for
internal evaluation of sulfation patterns within them for subsequent structure-activity studies.
Figure 1.9: Unsaturated disaccharides derived from CS by enzyme catalysed
elimination.
Abbreviation: R = SO3- or H .
Dermatan Sulfate
Chondroitin-6-Sulfate
Chondroitin-4-Sulfate
39
1.21 Glycosaminoglycans and cancer
Recent studies have demonstrated the significant roles played by GAGs and
proteoglycans in tumourigenesis and tumour progression (Yip et al, 2008 and Conte et al,
2007). For example, in breast cancer, changes in GAG and PG expression on the cell surface
and in the ECM allow tumour cells to proliferate, gain the ability to invade surrounding
tissues, metastasize to distant organs and induce angiogenesis (Guo et al, 2007 and Polyak,
2007).
HS are present on the surface of every eukaryotic cell, inclusive of both tumour cells
and the surrounding cells. This polymer has also been shown to be vital for tumour survival
(Liu et al., 2002). This includes the endothelial-cell compartment that is very close to a
growing tumour; indeed HS has been linked with the ability to modulate the process of
tumour angiogenesis (Gandhi and Mancera, 2010 and Ram et al, 2002). HS chains on the
tumour-cell surface have been proven to be important in many aspects of tumour phenotype
and development, including cellular transformation, tumour growth, invasion and metastasis
(Liu et al, 2002 and Sanderson et al, 2001). In vivo studies in mice highlight that changes in
the fine structure of tumour cell surface HS have marked effects on tumour cell growth
kinetics and metastasis formation (Liu et al, 2002). Some HS sequences expressed on the
tumour cell surface appear pro-tumourogenic, whereas others are anti-tumourogenic (Gandhi
and Mancera, 2010). Recent advances in structural elucidations of HS have led to the
discovery of its anti-tumourogenic capability both in vivo and in vitro (Gandhi and Mancera,
2008). HS structure-activity relationship studies, such as this have opened up many new
exciting avenues for the generation of polysaccharide-based anti-cancer therapeutics
( Linhardt 2013:Ram et al, 2002).
Changes in HS structure on the tumour cell surface seem to mediate their effects by
regulating differential growth-factor signaling, cell adhesion, proliferation and migration (Liu
40
et al, 2002 a). Moreover, alterations in the level of expression of the protein core of HSPGs as
well as HS structural differences and/or density on HSPGs, can potentially make cancer cells
highly versatile in the modulation of their behaviour (Esko and Lindhal, 2001: Tumbull et al,
2001).
The structural complexity of HS arises from the differential modification of individual
disaccharide units within an oligosaccharide chain (Esko and Lindhal, 2001: Tumbull et al
2001) which result ultimately in great structural diversity. One of the consequences of the
great structural diversity of HS structure is that these molecules are able to bind and interact
with a wide variety of proteins, such as growth factors, chemokines, morphogens, enzymes
and other signaling molecules, that are important for tumour development, such as FGFs.
Cells can perform subtle changes to the biosynthesis of HS chains and hence have the
ability to change how the cells interact with these molecular effectors that bind HS. This
allows the tumour cell HS-GAGs (both at the cell surface and extruded into the ECM) to
modulate directly several aspects of tumour-cell phenotype, including growth kinetics,
invasiveness and metastatic potential (Varki and Varki, 2002). One of the consequences of
tumour-derived HS or HSPG is that, it can be pro-tumourogenic or anti-tumourogenic
depending on whether it is anchored at the cell surface or present in the ECM as soluble-free
GAGs (Liu et al 2002), as well as depending on the HS-GAG sequence.
Recently, it has been demonstrated that cancer cells alter their cell-surface HS profile
during the process of transformation, including differential expression of particular
proteoglycan protein core sequences, in addition to changing the HS fine structure of given
proteoglycans (Blackhall et al 2001). Other studies have revealed that HS chains are involved
in the initial oncogenic transformation of a normal cell to a tumour-cell (Xiang et al, 2001:
Filmus 2001). Changes in both the expression level and the oligosaccharide sequence
characteristics of cell-surface HSPGs have been shown to correlate with transformation in
41
several malignancies (Ram et al, 2002). For example, the HSPG syndecans is required to
maintain the differentiated morphology and localisation of epithelial cells. Syndecan-1
expression is down regulated in various malignant tumours, including uterine carcinoma and
multiple myeloma (Ram et al, 2002). Its expression decreases as in situ carcinoma progresses
to invasive carcinoma (Sanderson 2001). This decrease in expression may be linked to
phenotype changes in these cancers. Specific HS structural changes have been noted during
malignant transformation of colon cancer cells from adenoma to carcinoma (Jayson 1998).
Likewise, glypican-1, another cell-surface HSPG that closely control cell growth and
division, has been shown to act as a negative regulator of cell proliferation for certain tumour
types ((Ram et al, 2002). Glypicans have also been shown to modify cellular responses to
bone morphogenetic proteins and insulin-like growth-factor-2 -factors that are important in
cellular division and differentiation (Ram et al, 2002). An association has also been made
between specific mutations in HS-related biosynthetic genes and inherited syndromes that
increase cancer risk, implicating these molecules in tumourigenesis (DeBaun et al, 2001).
Simpson–Golabi–Behmel syndrome (SGBS) is a complex congenital overgrowth syndrome
with features that include macroglossia, macrosomia, and renal and skeletal abnormalities, as
well as an increased risk of certain malignancies. Most cases of SGBS seem to arise as a
result of either deletions or point mutations within the gene that encodes glypican-3 (GPC3)
at Xq (Mundhenke 2002). GPC3 expression is also down regulated in a number of cancers,
including breast and ovarian carcinomas, and mesotheliomas (Mundhenke 2002).
Tumour cell surface HS also binds growth factors, cytokines and structural proteins
that are involved in modulating autocrine and paracrine signaling loops that are important for
tumour growth and progression (Mundhenke 2002) .The diverse structural characteristics of
HS enable them to act either as inhibitors or potentiators of these signalling loops, depending
42
on their sequence context (Liu et al, 2002). Recent studies have highlighted that, in vitro,
tumour cell surface HS can promote growth-factor signaling and tumour-cell proliferation.
Tumour cells are reported to influence actively the affinity of their HSPGs for FGF-2,
as well as for other growth factors, by modulating the overall density and sulfation pattern of
their HSPGs. Modified HS and CS, have been studied as potential cancer therapeutics. In an
attempt to generate a potentially therapeutic mimetic of syndecan-1, Pumphrey and
colleagues discovered that carbodiimide-modified glycosaminoglycans reduced breast cancer
and myeloma cell viability by inducing apoptosis (Pumphrey et al, 2002). Moreover,
modified CS abolished breast tumour growth in nude mice. HS mimetics with anti-cancer
properties such as KI-111 [2-(4-fluoro-3-nitro-benzoyl) benzoic acetic anhydride] inhibited
tumour-cell adhesion, migration, growth, and invasion in vitro (Ishida et al., 2004).
In contrast, other KI related compounds inhibited cancer invasion and migration but
promoted tumour cell adhesion (Ishida et al, 2004: Simizu et al, 2004).
HS has also been shown to be involved in the promotion and inhibition of tumour
angiogenesis with many approaches aimed at blocking the interactions between HS and
angiogenic growth factors (Sanderson. 2001).
1.22 Tumour angiogenesis
Angiogenesis is a natural process that involves both the growth of new blood vessels
from pre -existing vessels and also closely regulated sequence of events starting with the
degradation of the basement membrane by activated endothelial cells (Hussain et al 2009).
Tumours cannot grow as a mass above few mm in size unless a new blood supply is induced.
The various stages involved in tumour angiogenesis are illustrated in Figure 1. 10.
43
Angiogenesis is controlled by a balance between proangiogenic factor [including
FGFs: acidic (FGF-1) and basic (FGF-2), Vascular endothelial growth (VEGF), Tumour
necrosis factor-alpha (TNF-alpha), Follistatin Granulocyte colony-stimulating factors (G-
CSF), Hepatocyte growth-factor (HGF)] and anti-angiogenic factors [including anti-
angiogenic antithrombin III, CD 59 complement fragment, heparin hexasaccharide fragment,
human chorionic gonadotropin (hCG)]. The angiogenic switch represents the overall
activities of the angiogenic stimulators and inhibitors which may either shift the balance
towards inhibition or stimulation (Presta et al, 2003). Tumour neovascularization and angio-
proliferative diseases result in uncontrolled endothelial-cell proliferation.
HSPG’s participates in the modulation of the neovascularization that happens in
different physiological and pathological conditions. This modulation occurs through
interaction with angiogenic growth factors (Presta et al, 2003), which is due, in part, to their
capacity to bind to and modulate the activity of angiogenic growth factors. However
contrasting effects can be obtained depending on the types of HSPGs and/or on the
experimental conditions adopted e.g, purified perlecan enhances angiogenesis induced by
FGF-2 while other purified HSPGs are ineffective (Aziever et al, 1994). Glypicans support
the binding of FGF-1 and FGF-2 to human tyrosine kinase FGF receptor-1 (FGFR-1) in a cell
free system and replaces heparin in supporting FGF-2 induced cellular proliferation of HS-
negative cells expressing FGFR-1 (Bonneh-Barkay et al, 1997). Soluble heparin/HS inhibit
the binding of FGF-2 to FGFRs and HSPGs present on the surface of endothelial cells
(Coltrini et al, 1994). Thus, this observation suggest that negative effects on angiogenesis
may be exerted by the binding of angiogenic growth factors to soluble HSPGs or GAGs
rather than to cell-associated HSPGs.
44
HSPGs may also modulate angiogenesis also by protecting angiogenic growth factors
from heat (Gospodarowicz and Cheng, 1986) and proteolytic degradation (Coltrini et al,
1994) and by affecting their radius of diffusion (Flaumenhaft et al, 1989). Finally, HSPGs
present in the ECM may act as a reservoir for angiogenic growth factors that will reach
higher local concentrations and will sustain the long-term stimulation of endothelial cells
(Presta et al, 1989). A common theme among growth factors interacting with TK receptors is
the involvement of ligand-induced receptor dimerization in receptor activation (Ullrich and
Schlessinger, 1990).
Crystal structures of HS/FGF/FGFR ternary complexes revealed markedly different
geometrics (Pellegrini et al, 2000). A single molecule of heparin/HS may bind several
molecules of FGF-2 (Coltrini et al, 1993) suggesting that GAGs induce oligomerization of
angiogenic growth factors. Heparin has been reported to induce dimerization of FGF-2 in cell
free system (Coltrini et al, 1993). It has also been demonstrated that the dimerization and
activation of FGFR catalysed by heparin-dependent oligomerization of FGF is required to
induce a mitogenic response (Spivak-Kroizman et al, 1994). FGF-2 molecules has been
recently demonstrated to self-associate through specific interactions in a sequential pattern,
resulting to the formation of bioactive FGF-2 dimmers, and that Heparin can serve as a
platform to stabilize the inter-molecular FGF-2 interactions, thus favouring receptor
dimerization (Kwan et al, 2001). The capacity of various angiogenic factors to bind
heparin/HS indicates that molecules that are able to interfere with this interaction may act as
angiogenesis inhibitors; for example, the ability of low molecular weight heparin fragments
to be administered systemically in order to reduce the angiogenic activity of FGF-2 and
VEGF (Norrby 2000; Norrby and Ostergaard, 1997).
45
The biological activity of angiogenic growth factors on endothelial cells is controlled
by a complex interplay among free and cell-associated heparin/HS GAG chains. In this
scenario, natural and synthetic heparin related angiostatic compounds play their
pharmacological action (Presta et al, 2003). This observation indicates that distinct structural
requirements are necessary for the interaction of heparin/HS with different growth factors.
Even though these specific binding sequences may be masked in heparin due to its high
degree of sulfation, the high heterogeneity in HS structure allows a more refined tailoring of
selective binding regions that may influence the biological activity and bioavailability of
heparin/HS-binding growth factors (Presta et al, 2003).
46
Figure 1.10: Stages involves in tumour angiogenesis
47
1.23 Fibroblast growth factors (FGFs) and their receptors (FGFRs) in human breast
cancer
The pleiotropic effects of FGFs are mediated through four highly conserved receptor
tyrosine kinases (RTKs), known as FGF receptor 1-4 (FGFR1-4). The extracellular domain of
these receptors contains three immunoglobulin-like (Ig) domains (D1, D2 and D3) (Turner
and Gross 2010), which bind to specific members of the FGF family of growth factors.
The second and third Ig domains are the most important for FGF ligand binding and
specificity; whereas the first Ig domain, absent in certain isoforms, is presumed to have an
auto inhibitory function (Turner and Gross, 2010). Alternative splicing of the carboxyl half of
the third Ig domain yields either the IIIb or the IIIc isoforms of FGFR1-3 (Turner and Gross,
2010: Eswarakumar et al, 2005).These various isoforms of FGFRs exhibit tissue-specific
expression and respond to different spectrum of the 18 mammalian FGFs known to date
(Beenken and Mohammadi, 2009).
Many researchers have linked overexpression of FGFs to human breast cancer and this
finding has been substantiated by other in vitro studies which equally revealed multitudes of
properties that suggest their involvement in breast cancer induction, progression and
metastasis (Dickson et al 2000).
FGFR2-IIIb, expressed usually in epithelial cells, can be activated by FGFs of
mesenchymal origin e.g. FGF-7 and FGF-10, whereas FGFR2-IIIc e.g FGF-1 and
FGFR 2IIIc expressed on mesenchymal tissues responds to ligands secreted by epithelial
cells (Rusnati et al, 1994).
Studies have highlighted the critical role of aberrant FGFR2 signaling in cancer, including
overexpression of FGFR2 and its ligands, mutations and amplifications of the receptor, and
receptor isoforms switching (Turner and Gross, 2010: Eswarakumar et al, 2005). Single
nucleotide polymorphisms (SNPs) of FGFR2 correlate with increased risk of breast cancer
48
development, presumably due to elevated FGFR2 expression. Missense, potentially
activating, mutations of FGFR2 have been reported in multiple cancer types, including
endometrial, ovarian, breast, lung, and gastric cancer (Turner and Gross, 2010).
Furthermore, the FGFR2 gene is amplified in a subset of gastric and breast cancers
(Turner and Gross, 2010). The co-expression of FGFR-2IIIb and FGF7, in pancreatic and
gastric cancers, as well as lung adenocarcinomas, is associated with poor prognosis (Turner
and Gross, 2010), which may likely due to aberrant receptor activation through the formation
of autocrine activation loop. However, decreased expression of FGFR-2IIIb has been
reported in several cancer types during tumour progression and phenotypic change. (Turner
and Gross, 2010), possibly reflecting the physiological role of FGFR2 in regulating tissue
homeostasis.
A number of FGF family members and their receptors have been detected in both
normal and malignant breast tissue through the application of reverse transcription
polymerase chain reaction procedures (Matsuike et al, 2001). Increased expression of
FGFR2-IIIb has been described in breast, colorectal, cervical, pancreatic and prostate
cancers; however, it may also act as a tumour suppressor (Turner and Gross, 2010). Hence,
interactions between GAG mediated growth-factor binding to these TK receptors has the
potential to modify the growth and metastatic potential of tumours, which may enable new
treatments for the growth and progression of solid tumours in the future.
49
1.24 The cell cycle
Figure 1.11: The cell cycle showing the two major events that takes place within the cell.
Control of the cell cycle is an extremely complex process that networks with
numerous regulatory proteins, which control the events leading ultimately to proliferation,
cell growth, organism development, regulation of DNA damage repair and diseases, such as
cancer. The cell cycle can be divided into two major sections as illustrated in the diagram
above (Figure 1.11). These are: Interphase, the non-dividing but metabolically active period
of the cell cycle including Gap I (G1), DNA Synthesis (S), Gap (G2) and the Mitosis phase,
G2 Phase G1 Phase
G0 Phase
S Phase
M Phase
50
comprising prophase, metaphase, anaphase, and talophase. (Peng 1998: Rickert 1996 and
Roy 1994). G1 and G2 phases of the cycle represent the gaps between the two major events
that occur in the cell i.e. synthesis and mitosis.
The G1 phase is the first gap in the cycle in which the cell is preparing for synthesis of
DNA (replication) and is also a growing stage for the cell. S-phase is the first major events in
the cell cycle in which the cell starts synthesising new DNA. During the S-phase the new
daughter strands of DNA for each chromosome is synthesised and as a result of this DNA
replication, each chromosome gains a second chromatid, hence, duplication of genomic
information takes place (Johnson and Walker, 1999).
The G2 phase is the second gap in the cell cycle that occurs before the cell progress to
mitosis and follows the DNA synthesis phase. During the G2 period of growth, materials are
prepared for the next mitotic division. At this stage, the cell regulatory proteins check the
entire cascade involved at the S-phase before the cell cross to this phase and if everything
iscorrect, then the cell can progress to the next phase which is mitosis. The mitotic phase is
where the actual cell division takes place through a cascade of events, as presented in the
diagram below (Figure 1.12). Successful completion of mitosis leads to an onset of interphase
and the cell begins a period of growth which spans through the first phase, called G1 and
continues through the S and G2 phase. However, new cells generated from this series of
events could either start a new cycle or remain in a state of quiescence known as G0. G0 is a
gap between mitosis and interphase. At this stage, the cell is inactive and no physiological
growth is occurring; however, the cell has the potential to grow if the checkpoints adequately
allow it.
51
Figure 1.12: The four stages of mitosis
The cell cycle is a continuous event in both normal and cancer cells, including breast cancer. All the
cell cycle events are strictly controlled by the regulatory proteins in order to control growth and development.
However, there is uncontrolled and increased proliferation in cancer cells, especially breast cancer cells. This is
probably a result of the impairments of some of the regulatory proteins that control or check abnormal
proliferation. Some of these proteins are given in Figure 1.13
52
1.25 Cell Cycle regulation
Figure 1.13: The cell cycle and its regulation by cyclins, CDKs, and CDKIs.
The cell cycle is divided into four distinct phases (G1, S, G2, and M). The progression of a cell through the cell
cycle is promoted by CDKs, which are positively and negatively regulated by cyclins and CDKIs, respectively.
As shown, cyclin D isoforms (cyclin D1–D3) interact with CDK4 and CDK6 to drive the progression of a cell
through G1. The association of cyclin E with CDK2 is active at the G1-S transition and directs entry into S-
phase. S-phase progression is directed by the cyclin A/CDK2 complex, and the complex of cyclin A with Cdc2
(also known as cdk1) is important in G2. Cdc2/cyclin B is necessary for the entry into mitosis. The INK4 (for
inhibitor of cdk4) class of CDKIs, notably p16lnk4a
, p15lnk4b
, p18lnk4c
, and p191nk4d
, bind and inhibit cyclin
D-associated kinases (CDK4 and CDK6). The kinase inhibitor protein group of CDK inhibitors, p21waf1
, p27kip1
,
and p57kip2
, negatively regulate cyclin E/CDK2 and cyclin A/CDK2 complexes.
53
The cell cycle is regulated strictly at selected checkpoints that are controlled by group
of modulators known as cyclin and cyclin-dependent kinases (CDKs), cyclin-dependent
inhibitors (CDKI) and retinoblastoma gene products (pRB). These modulators are the key
regulatory factors that dictate the orderly progression of the cell cycle through the activation
and deactivation processes (Johnson and Walker, 1999). A number of CDKs have been
identified including CDKs A, B1, B2, C, D1, D2, D3, E and many more (Figure 1.13). All
cyclins contain a cyclin box, an important domain used to bind and activate CDKs. Cyclins
and CDKs are also involved in the regulation of cell transcription, DNA repair,
differentiation, and apoptosis (Peng 1998: Rickert 1996 and Roy 1994). Phosphorylation of
CDK subunits can both positively and negatively regulate kinase activity (Arellano 1997) and
ubiquitin-mediated proteolysis plays another crucial role in cell cycle control by targeting
cyclins and other regulators for destruction at key times during the cell cycle (King 1996 and
Pagano 1997). Some CDK’s have been reported by LaBaer and co-workers to positively
regulate the cell cycle by functioning as assembly factors for cyclin D/cdk complexes
(LaBaer et al, 1997). CDK’s are regulated by several methods, one of which includes
phosphorylation of threonine and tyrosine residue. CDK’s are very important to cell cycle
control because its deactivation will prevent mitosis, which is the ultimate committal event in
the cell cycle (Johnson and Walker, 1999).
1.26 Role of Cell-cycle Regulatory molecules in Breast Cancer Development and
Progression
The resulting DNA damage and the integrity of mitotic spindles caused by any
intrinsic or extrinsic elements are assessed during transition between the four major phases of
the cell cycle. Cell cycle progression is arranged by the relative activity of a family of serine
54
threonine kinases (Figure 1.14). The cyclins encode co-regulatory subunits of a holoenzyme
that phosphorylates and inactivates a number of substrates including pRb (Hilakivi-Clarke et
al, 2004). Cyclin D1 has been reported to be one of the commonly over expressed genes in
breast cancer (Arnold and Papanikolaou, 2005: Sutherland and Musgrove, 2004). Oestrogen
receptor (ER)-positive breast cancers has also been shown to produce cyclin D1 amplification
and over expression more commonly than ER-negative cancers, and it is in the ER-positive
subgroup that the most consistent association between cyclin D1 amplification and poor
outcome has been found (Sutherland and Musgrove, 2004). Sutherland and others have
suggested that the ability of cyclin D1 to modulate transcription may be important in
mammary oncogenesis (reviewed in Arnold and Papanikolaou, 2005: Sutherland and
Musgrove, 2004)
1.27 Cyclin D1
Cyclin D1 encodes the labile regulatory subunit of the cyclin CDK4/6 holoenzyme.
Phosphorylation of the pRb protein is thought to change the confirmation of pRb which, in
turn, alters further upon phosphorylation by cyclin E/CDK2 complexes. It is considered that
the phosphorylation of the pRb protein by the cyclin D1/CDK4/6 holoenzymes is required for
transition through the G1 /S-phase of the cell cycle. The cyclin D1 gene has been reported by
Zwijsen and his co-workers to physically associate with the ER and induce ER signaling in a
CDK-independent manner (Zwijsen et al, 1997).
Immuno-neutralizing experiments performed by Lukas et al have revealed that cyclin
D1 is required for oestrogen-induced cellular proliferation (Lukas et al, 1996). It has also
been shown to enhance ER signaling through functioning as a coactivator-like protein,
55
analogous to the p160 steroid receptor coactivator (SRC) of the ER, in cultured cells.
Research has revealed that up to 30- 50% overexpression of Cyclin D1 is present in primary
breast cancers, partly due to amplification of the cyclin D1 gene, CCND1; hence, cyclin D1 is
one of the most commonly overexpressed oncogenes in breast cancer (Arnold and
Papanikolaou, 2005: Sutherland and Musgrove, 2004). This overexpression effect of Cyclin
D1 is more pronounced in ER-positive breast cancers than ER-negative cancers, and it is in
the ER-positive subgroup that the most consistent association between cyclin D1
amplification and poor outcome has been reported (Sutherland and Musgrove, 2004).
In addition, Cyclin D1 has been proven to be overexpressed in ductal hyperplasia and
ductal carcinoma in situ as well as invasive cancers and these findings suggest that it may
play a role in the evolution of breast cancer. In contrast to general opinion based on this
finding that cyclin D1 overexpression might be expected to be associated with high
proliferation rates, over expression of cyclin D1 in breast cancer is characteristic of slow-
growing, more differentiated cancers (Sutherland and Musgrove, 2004).
Moreover, in a panel of breast cancer cell lines, CDK4 activity was not strictly related
to cyclin D1 expression, suggesting that functions of cyclin D1 other than its ability to
activate CDK4 and promote cell proliferation might contribute to its activity as a mammary
oncogene ( Fu et al, 2004: Sutherland and Musgrove, 2004). Amplification of the cyclin D1
gene, CCND1, is observed in just a few of cyclin D1 overexpressing breast cancers.
Furthermore, Cyclin D1 has been implicated in the oncogenic actions of Ras and Neu/erbB2
Murine mammary tumours induced by oncogene display increased expression of cyclin D1,
while cyclin D1 expression is necessary for Ras or erbB2-mediated mammary tumourigenesis
(Sutherland and Musgrove, 2004). However, the relationship between cyclin
56
D1overexpression and erbB2 amplification in human breast cancer is yet to be elucidated
(Arnoldand Papanikolaou, 2005).
1.28 Cyclin E1
Cyclin E1 is reportedly overexpressed frequently in breast cancers, particularly ER-negative
breast cancers. This observation is attributed to the presence of a number of low molecular
weight isoforms, which appear to contribute to poor clinical outcomes (Sutherland and
Musgrove, 2004). The low molecular weight isoforms display enhanced binding to CDK2 to
produce a complex that is relatively resistant to inhibition by p21 and p27 (Wingate et al,
2005). Moreover, cyclin E1 overexpression is of greater prognostic significance when p27
expression is reduced and CDK2 activation increased (Caldon et al, 2010). The association
between cyclin E1 overexpression and markers of proliferation together with the above
mentioned role as suggested by Caldon and co-workers that the CDK dependent functions of
cyclin E1 may be critical to its role in mammary oncogenesis (Caldon et al, 2010).
1.29 p27 and p21
These two genes are tumour suppressor genes and many studies have confirmed this
(Musgrove 2004). The role of p21 and its abundance as a modulator of outcome in primary
breast cancer is still unclear. Expression is generally undetectable in normal breast epithelial
cells and very variable in breast cancers, with conflicting data on the prognostic implications
of p21 expression from a limited number of small patient groups (Tsihlias et al, 1999).
57
The use of p27 as a prognostic marker has been more widely investigated. Normal human
mammary duct epithelial cells exhibit nuclear immunoreactivity for p27, while breast cancers
often exhibit reduced p27 expression and/or mislocalisation of p27 to the cytosol (Alkarain et
al, 2004). In general, reduced nuclear p27 expression is associated with high tumour grade
and ER negativity, and in a small majority of studies, represents an independent prognostic
indicator upon multivariate analysis (Alkarain et al, 2004). However, loss of heterozygosity
at band 13 of chromosome 12, which harbours the p27 gene, has been reported in breast
cancers, although, somatic mutations in this gene are rare (Alkarain et al, 2004), and the
predominant mechanism for loss of protein expression appears to be linked to increased
protein turnover. Newman and Spataro have reported that ErbB2 overexpression associates
with low p27 levels in breast cancer patients overall (Newman et al, 2001) or in the
lymphnode negative subset (Spataro et al, 2003). Hence, activation of signaling pathways
downstream of this receptor may promote p27 degradation. However, RTK signaling can also
lead to restriction of p27 to the cytosol. Additionally, in cancers with either low or high p27
expression, the presence of cytosolic p27 was associated with worse overall survival rate
(Alkarain et al, 2004).
1.30 Therapeutic target in breast cancer
There are two major therapeutic approaches that are useful in the treatment of breast
cancer; namely: the modulation of the cell cycle and direct inactivation of checkpoint
controls. The following section explores the recent evidence that validates this type of clinical
intervention.
58
1.31 Modulation of the cell cycle
Alteration to any of the major phases of the cell cycle may lead to carcinogenesis,
which is a major concern in the field of cancer research. Subsequently, the cell cycle has
become the bedrock of the major therapeutic interventions research, providing numerous
opportunities to target checkpoint controls in order to develop new therapeutic strategies for
combatting this disease.
These include induction of checkpoint arrest leading to cytostasis and, ultimately, apoptosis;
arrest of proliferating cells in defined stages of the cell cycle, which may in turn sensitize
them to treatment with other therapeutic agents, such as radiation; and targeting therapies
towards specific regulatory components of the cell cycle (Caldon et al, 2010). Those drugs
that have diverse mechanisms of action and ex-chromosome breakage can cause cell cycle
arrest at both the G1/S and G2/M checkpoints (Lowe et al, 1993).
The most common and reliable chemotherapeutic approach is the induction of DNA
damage, followed dogmatically by induction of apoptosis. Some chromosome breakers and
DNA cross links agents such as cisplatin and Mustard have been reported to cause cell cycle
arrest at both G1/S and G2/M checkpoints (Lowe et al 1993). G1 arrest caused by these
agents is mediated by p53, which in turn induces an increase in p21, resulting in inhibition of
cyclin/CDK2 and cyclin/CDK4 complexes and hypophosphorylation of Rb (Robert and
Thompson, 1979). Up-regulation of p21 also results in sequestration of PCNA, which
contributes to arrest at G1/S. The G2/M checkpoint induced by DNA damage can occur by
either p53-dependent or independent mechanisms (Paules et al, 1995: Agawal et al, 1995).
Both p21 and phosphorylation of CDK1 is required for passage of cell from G2 phase into M-
phase and can participate in the DNA damage G2/M checkpoint. Tumour cells in which p53
are inactive can bypass the G1/S checkpoint and exhibit increased sensitivity to DNA-
59
damaging agents such as cisplatin (Fan et al, 1997) as a result of failure to arrest and repair
their damaged DNA.
Another intervention is also made possible by the use of microtubular inhibitors such
as taxol and vinca alkyloids. These act principally by distrupting the normal tubular
polymerisation/depolymerisation and mitotic spindle formation (Gorbsky 1997). Hence, the
cells are forced either to initiate a p53-dependent arrest at the mitotic spindle assembly
checkpoint (Cross et al., 1995), a radiosensitive phase of the cell cycle, or continue to
progress through M-phase and become aneuploid and arrest in G1 (Argawa, 1995).
Arrest in G2/M induced by these drugs (taxol and vinca alkaloids) is associated with
stabilization of cyclin B complexes (Poon et al, 1997). Tumour cells treated with microtubule
inhibitors can undergo apoptosis from both G1 and G2 arrest (Wood et al, 1995). Microtubule
inhibitors have also proven effective in the clinic as radiosensitizers (Liebmann et al, 1994).
Combined chemotherapy/radiotherapy with taxol, which blocks cells at the mitotic spindle
assembly checkpoint, can enhance the sensitivity of radiation-resistant tumours to
radiotherapy (Liebmann et al, 1994: Tischler et al, 1992).
G1 checkpoint arrest can also be triggered by depletion of ribonucleotide pools,
caused by nucleoside analogs such as hydroxyurea and gemcitibine. G1 arrest at a point may
be totally distinct from that associated with DNA damage (Linke et al, 1996).This latter G1
checkpoint is mediated by p53 and also requires up-regulation of p21 (Wharl et al,1997). In
checkpoint-defective cells, such as those with inactive p53, bypass of the G1/S checkpoint
produces DNA strand breaks, resulting in cell death (Chang et al, 1998). Both gemcitibine
and hydroxyurea have also been effectively used as radio sensitizers for a variety of tumour
types (Shewach and Lawrence, 1996). Anti-metabolites such as methotrexate and 5-
fluorouracil have been reported to inhibit thymidylate synthase and DNA synthesis and
60
induce a p53-dependent S-phase arrest (Matsui et al, 1996). However in tumour cells, in
which p53 is inactive, DNA damage induced by these drugs goes undetected and cells
progress to G2 and subsequently undergo apoptosis (Lowe et al, 1993).
These drugs are also used clinically as radiosensitizers as a result of their ability to
arrest cells in the radiosensitive phase of the cell cycle (Robertson et al, 1996).
Topoisomerase inhibitors have been reported to also cause DNA damage, resulting in
increased levels of cyclin A and S-phase arrest or inactivation of cyclin B/CDK2 complexes
and G2/M arrest (Kaufmann et al, 1999). Moreover, the prominent role of p53/p21-mediated
activity for many of the above-named drugs in addition to the activity of topoisomerase
inhibitors can also be mediated by the Rb/p16 pathway. In some cell types, drugs such as
camptothecin and etoposide produce an increase in p16, which inhibits phosphorylation of Rb
resulting in a G1 cell cycle arrest (Shapiro, 1998).Therefore, in addition to p53; their activity
may also be dependent on the presence of a functional Rb protein. Tumour cells that lack
functional Rb can bypass this checkpoint and progress through the cell cycle, becoming
genetically unstable and acquiring additional genetic alterations including changes in ploidy.
1.32 Direct inactivation of checkpoint controls
Some successful or potentially successful therapeutic strategies involve the use of agents that
target cell cycle regulatory molecules. As mentioned previously, the activity of cyclin-kinase
complexes is regulated by phosphorylation and several CDK inhibitors have been identified,
which exhibit specificity for the ATP-binding pocket of these and block their phosphorylation
CDKs (Walker et al, 1998). Chemical inhibitors of CDKs such as olomoucine and its analog
61
roscovitine exhibit specificity for CDK1 and CDK2 (Vesely, 1994). These inhibitors can
induce both G1 and G2 arrest as well as apoptosis (Walker, 1998).
As mentioned above, in response to DNA-damaging agents, some tumour cells can
arrest in G2 in a p53-independent manner. This G2/M checkpoint arrest occurs as a result of
phosphorylation and inactivation of CDK1. Staurosporine and its second-generation analog
7-hydroxystaurosporine (UCN-01) inhibit the phosphorylation of CDK1, resulting in the
activation of this M-phase regulator and abrogating the G2/M arrest (Wang et al,1996). Use
of UCN-01 has been most successful in combination with DNA-damaging agents such as
cisplatin (Bunch and Eastman, 1996) and camptothecin (Shao et al,1997) in p53- deficient
cells that can bypass the G1 checkpoint and would otherwise arrest in G2. As a consequence
of UCN-01 treatment, tumour cells that have sustained DNA damage progress through the
cell cycle beyond the G2/M checkpoint and undergo apoptosis (Wang et al, 1995). Similar
strategies with several agents (such as caffeine) that abrogate the G2 checkpoint by activating
CDK1 have been shown to preferentially sensitize p53-deficient cells to other genotoxic
agents such as radiation and etoposide (Yao et al, 1996).
Active cyclin D-kinase complexes, which serve to phosphorylate Rb and release E2F,
can also be inhibited by small peptides derived from p16 (Fahraeus et al, 1998). A 20-amino-
acid peptide of p16 can bind CDK4; inhibit activation of cyclin D-CDK4 activity, and block
cell cycle progression through G1. As predicted, this cell cycle arrest requires a functional Rb
protein (Fahraeus et al, 1998). Similarly, double-stranded DNA with high affinity for E2F can
act as a molecular decoy, compete for E2F binding to DNA, and inhibit the ability of E2F to
regulate target genes such as cdc2 (CDK1) and cyclin E (Bandara et al, 1997: Morishita et al,
1995).
62
Targeting of breast cancer by anti-angiogenic drugs available to date have been shown
to be a failure and regulators of the cell cycle in conjunction with radiotherapy and surgery
are still the mainstay in the treatment of the disease. However, during the next 20 years more
targeted therapy is likely to become the preferred method of treatment. It is hoped that the
results shown in this study could lead to a new class of targeted cancer therapeutics aimed
solely at the treatment of breast cancer.
63
1.33 Cell death
Natural death is an integral part of cell development and this was also described by
Cotter and Curtin as a natural event that can be related to an integral part of toad development
(Cotter and Curtin, 2003). Natural death has been described newly in many ways after this
observation. There are two major mechanisms by which cells undergo natural death: necrosis
or apoptosis.
1.34 Necrosis
Necrosis, otherwise known as cell murder, is described as the death of cells through
external damage (extrinsic factors), usually caused by destruction of the plasma membrane or
the biochemical pathways that support the cells integrity. The necrotic cell is characterised by
swollen morphology and plasma membrane lyses, which releases cytoplasmic components
(necrotic debris) into the surrounding tissue spaces, attracts inflammatory cells and ultimately
leads to the tissue destruction characteristic of inflammation. The death of a single cell by this
mechanism might be resolved in some tissues, but a large number of cells dying by necrosis
usually results in inflammation, subsequent repair and scarring; leading to compromise and
permanent alteration of tissue architecture.
Necrosis can occur in a matter of seconds (Collins et al, 1997) and also can cause loss
of cell-membrane integrity followed by swelling of both cytoplasm and mitochondria;
ultimately resulting to cell and many of its internal organelles lyses’ (Leist and Jäättelä,
2001). The products of necrotic cells are usually phagocytosed by macrophages, and this
process provokes an inflammatory response in vivo. Necrosis-like programmed cell death
describes programmed cell death that does not involve chromatin condensation and has
64
varying degrees of other apoptotic features. In some cases caspase-1 and caspase-8 have been
implicated in this type of programmed cell death (Leist and Jäättelä, 2001). Some of the
factors that lead to necrosis are detailed in the following sections.
1.35 Pathophysiology and physiological factors leading to necrosis
Cell and tissue death is a common phenomenon that usually arises suddenly as a result
of some extreme conditions (high temperature, heat shock etc): a process that leads to
unregulated process of both membranes and cytosol destruction. This finding led to the
concept that when cell destruction is followed by rapid disruptions of the plasma membrane,
cytoplasmic structures, and the nucleus, death is passive and unregulated. However, necrotic
cell death could also be regulated by some specific physiological conditions such as bacterial
infections, viral infection, bacterial toxins etc. (Warny et al, 2000: Dong et al, 1997).
Necrosis can also be triggered by components of the immune system, such as
complement (Shimizu et al, 2000), activated natural killer cells (Blom et al, 1999), and
peritoneal macrophages (Arantes et al, 2000).The pathogen-induced necrotic programs in
cells of immunological barriers (e.g. intestine mucosa) may reduce invasion of pathogens
through the surfaces affected by inflammation (Ehlers et al, 1999).
Necrotic cell death can also result from pathological conditions that are characterised
by inadequate secretion of cytokines, nitric oxide (NO) and reactive oxygen species (ROS). A
classic example of necrotic conditions is ischemia that leads to a drastic depletion of oxygen,
glucose, and other trophic factors and evokes massive necrotic death of endothelial cells and
non-proliferating cells of surrounding tissues (neurons, cardiomyocytes, renal cells, etc.)
(Elmore, 2007).
65
1.36 Apoptosis
Apoptosis is a form of cell death that usually occurs when cell is exposed to
unfavourable conditions such as heat, hypoxia, and radiation, cytotoxic anti cancer drugs,
toxicants or any physical damage (Elmore 2007). It is usually initiated in order to prevent
inflammation associated with necrotic process by a careful removal of damaged cells from
injury sites (Fin et al, 2005). Initiation of apoptosis triggers a series of events that culminate
in the cell’s destruction. This process is usually called "programmed cell death" as it is an
innate response of the cell that protects the remainder of the organism from a potentially
harmful agent (Wyllie et al, 1980). The process of apoptosis is illustrated in the diagram
below.
66
Figure 1.14: The processes involved in apoptosis
67
Apoptosis also describes a common mechanism by which cell undergoes natural
death. It involves cascades of preprogrammed arranged events, including morphological and
biochemical changes, which qualifies it as an example of programmed cell death (Wyllie et
al, 1980). During the initial phases of apoptosis, cells shrink and their nuclei condense, after
which they disintegrate into well-enclosed apoptotic bodies (Figure 1.14). The common
features of apoptosis include cell shrinkage, plasma membrane blebbing, cell detachment,
externalization of phosphatidylserine, nuclear condensation and ultimately DNA
fragmentation (Brauchle et al., 2014: Majno and Joris, 1995).
Apoptosis is a normal occurrence during development and aging and as a homeostatic
mechanism to maintain cell populations in tissues: it also occurs as a defence mechanism,
such as in immune reactions or when cells are damaged by disease or noxious agents
(Norbury and Hickson, 2001). However, many stimuli and conditions including physiological
and pathological are among other factors that triggers apoptosis; yet not all cells will
necessarily die in response to the same stimulus. At low doses, irradiation or some cytotoxic
drugs used for cancer chemotherapy results in DNA damage in some cells, ultimately,
leading to apoptotic death through a p53-dependent pathway (Elmore, 2007). Some cells
express Fas (Fatty acid synthetase) or TNF (Tumour necrosis factor) receptors that can lead
to apoptosis via ligand binding and protein cross-linking. Other cells have a default death
pathway that must be blocked by a survival factor such as a hormone or growth-factor
(Elmore, 2007).
Apoptosis and necrosis can occur independently, sequentially and simultaneously, but
there is need to make a clear distinction between the two processes
68
(Zeiss 2003: Hirsch 1997 ); the type of stimuli and/or the degree of stimuli play a critical role
in this process. Interestingly, low doses of some environmental perturbations such as heat,
radiation, hypoxia and cytotoxic anti-cancer drugs can induce apoptosis but these same
stimuli can result in necrosis at higher doses. In addition, apoptosis is a coordinated and often
energy-dependent process that involves the activation of a group of cysteine proteases called
“caspases” and a complex cascade of events that link the initiating stimuli to the final demise
of the cell (Elmore, 2007: Fin et al 2005). Apoptosis can also be seen as a stage-dependent
process from its induction to early, intermediate and late-stage apoptotic events (Figure 1.15
A-D)
69
Figure 1.15: Stages of apoptosis
(A) Full blown apoptotic Figure (early apoptosis); (B) Different forms of chromatin aggregation
(intermediate/mid apoptosis); (C) Late stage of apoptosis; (D) Very late apoptosis.
A B
C D
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1.37 Morphology of Apoptosis
There are various morphological changes that occur during apoptosis and some of
these changes were characterised by nuclear and cytoplasmic condensation, and cellular
fragmentation into membrane-bound fragments. Early apoptosis is usually characterised by
cell dehydration followed by changes in cell size and shape, resulting into smaller, dense
cytoplasmic and more tightly packed organelles cells (Fink and Cookson 2005). The
membrane bound fragments or apoptotic bodies (Figure1.16C) are consequently engulfed by
microphages, parenchyma cells, or neoplastic cells and are desolved within the
phagolysosomes (Figure 1.16D). This process allows cell deletion with little tissue disruption
and no inflammation.
The process of apoptosis and removal of apoptotic cells are practically free of
inflammatory reaction. Lockshin and William suggested this process of tissue deletion
without inflammation allows reutilization of cellular components (Lockshin and William,
1965). The morphological characteristics of apoptosis were purported to result from a general
mechanism of controlled cell deletion, which plays a complementary role to mitosis and
cytokinesis in maintaining stable cell populations within tissues. The concept of apoptosis
furthered the hypothesis that living cells are programmed genetically to contain components
of a metabolic cascade that, when activated, can lead to cellular death (Lockshin and Zakeri,
2001).
Various morphological changes that occur during apoptosis can be measured by
scatter light analysis (flow cytometry) and some of these changes are characterised by some
of the features described above. In short, the cells traversing through the focus of a laser
beam in a flow cytometer scatters the laser light. Analysis of the degree of scattered light
71
gives indepth information about the morpholical changes that characterise the onset of
apoptosis (Darzynkiewicz et al 1992).
Hacker also described the various morphological changes that occur in apoptosis by
light and electron microscopy (Hacker, 2000). Cells view under the electron microscope
shows cell shrinkage and pyknosis as the major morphological changes that characterised
early stage of apoptosis (Kerr et al., 1972). On histologic examination with haematoxylin and
eosin stain, apoptosis involves single cells or small clusters of cells. The apoptotic cell
appears as a round or oval mass with dark eosinophilic cytoplasm and dense purple nuclear
chromatin fragments (Figure 1.16 A). Electron microscopy also shows other subcellular
changes that occur during early chromatin condensation and some of these changes involve
aggregation of electron-dense nuclear material under the nuclear membrane although there
can also be uniformly dense nuclei (Figures 1.16 B). This process leads to extensive plasma
membrane blebbing followed by karyorrhexis and separation of cell fragments into apoptotic
bodies during a process called “budding.” The organelle integrity is still maintained and all of
this is enclosed within an intact plasma membrane. Macrophages that engulf and digest
apoptotic cells are called “tingible body macrophages” and are found frequently within the
reactive germinal centers of lymphoid follicles or occasionally within the thymic cortex. The
tingible bodies are the bits of nuclear debris from the apoptotic cells. The anti inflammatory
activity associated with both apoptosis process and removal of apoptotic bodies is due to the
following reasons: (1) apoptotic cells do not release their cellular constituents into the
surrounding interstitial tissue; (2) they are quickly phagocytosed by surrounding cells thus
likely preventing secondary necrosis; and (3) the engulfing cells do not produce anti-
inflammatory cytokines (Kurosaka et al, 2003: Savill and Fadok, 2000).
72
Figure 1.16: Morphology of apoptosis.
(A) Normally shaped nuclei (B) Chromatin clumping in apoptotic nuclei (C) Different features of
chromatin clumps (D) Chromatin superaggregation.
A B
C D
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1.38 Biochemical features of apoptosis
Apoptotic cells have been described previously as exhibiting several biochemical
modifications, such as protein cleavage, protein cross-linking, DNA breakdown, and
phagocytic recognition that together result in the distinctive structural pathology (Hengartner
2000). There are various biochemical features that ensue once apoptosis programme has been
initiated and some of these biochemical features are discussed below;
1.39 Activation of caspases
Activation of caspases is one of the biochemical features of programme cell death. This
process is trigerred by some of the external stimuli that causes apoptosis. Caspases are
usually expressed widely in an inactive proenzyme form in most cells: activation of this
proenzymes lead to casdade of events including activation of other procaspases, initiation of a
protease cascade, aggregation and autoactivation of other procaspases. This cascade of events
amplifies the apoptotic signaling pathway; thus leading to rapid cell death (Figure 1.17).
Caspases have proteolytic activity and are able to cleave proteins at aspartic acid residues,
although different caspases have different specificities involving recognition of neighbouring
amino acids. Once caspases are activated, there appears to be an irreversible commitment
towards cell death (Elmore 2007).
Ten major caspases have been identified and categorised broadly into initiators
(caspase-2,-8,-9,-10) (Cysteinyl aspartic acid-protease-2-8-9-10), effectors or executioners
(caspase-3,-6,-7) (Cysteinyl aspartic acid-protease-3-6-7) and inflammatory caspases
(caspase-1,-4,-5) (Cysteinyl aspartic acid-protease-1-4-5) (Cohen, 1997; Rai et al, 2005).
Other caspases such as caspase-11 (Cysteinyl aspartic acid-protease-11), have been shown to
74
regulate apoptosis and cytokine maturation during septic shock and caspase-12 (Cysteinyl
aspartic acid-protease). This mediates endoplasmic-specific apoptosis and cytotoxicity by
amyloid-β has been reported (Kang et al, 2002: Koenig et al, 2001: Nakagawa et al, 2000: Hu
et al, 1998). Extensive protein cross-linking is another characteristic of apoptotic cells, which
is achieved through the expression and activation of tissue transglutaminase (Nemes et al,
1996).
75
Figure 1.17: Activation of apoptosis signalling pathway
76
1.40 DNA fragmentation
DNA fragmentation is one of the earliest recognizable changes that characterised
irreversible commitment to programmed cell death (Wyllie 1980). This process is initiated by
breakdown effect caused by Ca2+
-and Mg2+-
dependent endonucleases, resulting in DNA
fragments of 180 to 200 base pairs (Bortner et al, 1995). Oberhammer and co workers have
reported that formation of the larger DNA fragments is unconnected to oligonucleosome
formation (Oberhammer et al., 1993). Similarly, cleavage of DNA into these larger fragments
is sufficient to allow chromatin condensation and subsequent apoptosis, without
oligonucleosome formation. DNA fragmentation can be clearly seen when the sample are run
on agarose gel electrophoresis and stained with ethidium bromide: a characteristic ladder
pattern is evident when viewed under UV light (Allen et al 1997).
1.41 Phosphatidylserine (PS) Translocation
Translocation of PS is another biochemical changes that takes place during early
apoptosis (Allen et al 1997). Bratton and co-workers described this biochemical feature of
apoptosis as the expression of cell-surface markers that result in the early phagocytic
recognition of apoptotic cells by adjacent cells, permitting quick phagocytosis with little
compromise to the surrounding tissue. This is achieved by the movement of the normal
inward-facing phosphatidylserine of the cell’s lipid bilayer to expression on the outer layers
of the plasma membrane (Bratton et al, 1997). Although externalization of phosphatidylserine
is a popular identified ligand for phagocytes on the surface of the apoptotic cell, however,
recent studies have shown that other proteins like annexin1and calreticulin are also exposed
on the cell surface during apoptotic cell clearance.
77
Annexin V, an anticoagulant with other biological effects, is a member of a family of
proteins which exhibits Ca2+
-dependent binding to negatively charged phospholipids (Allen
et al 1997). Annexin V binds strongly and specifically to phosphatidylserine residues and can
be used for the detection of apoptosis (Allen et al 1997). Externalisation of PS occurs in early
apoptosis when membrane integrity is still intact: this process make flow cytometric analysis
using fluorescein isothiocyanate- (FITC) labeled annexin V a useful quantitative measure of
early apoptosis; this method has also been used with the DNA intercalating dye PI. During
apoptosis the cells become reactive with annexin V after the onset of chromatin condensation
but prior to the loss of the plasma membrane (Arur et al, 2003). Annexin V binding has been
shown to reveal a much higher level of cells committed to apoptosis than PI staining,
However, PI staining enter necrotic cells while apoptotic cells are excluded (Allen et al
1997). Calreticulin is a protein that interacts with LDL (low density lipoprotein)- receptor-
related protein on the engulfing cell and is suggested to cooperate with phosphatidylserine as
a recognition signal (Gardai et al, 2005). The adhesive glycoprotein, thrombospondin-1, can
be expressed on the outer surface of activated microvascular endothelial cells and, in
conjunction with CD36 (Cluster of differentiation 36), caspase-3-like proteases and other
proteins, induce receptor-mediated apoptosis (Jimenez et al, 2000).
1.42 Mechanisms of apoptosis
The mechanisms of apoptosis have been described as a complex and sophisticated processes
involving energy-dependent cascade of molecular events (Figure 1.18). There are two major
mechanisms by which cells commit suicide by apoptosis, namely the extrinsic or death-
receptor pathway and the intrinsic or mitochondrial pathway (Figure 1.18). However, Igney
78
and Krammer have recently shown that the two pathways are linked and that molecules in
one pathway can influence the other (Igney and Krammer, 2002). There is also an additional
pathway known as perforin/granzyme which involves T-cell mediated cytotoxicity and
perforin-granzyme-dependent killing of the cell. The perforin/granzyme pathway can induce
apoptosis via either granzyme B or granzyme A (Elmore 2007).
The extrinsic, intrinsic, and granzyme B pathways converge on the same terminal
otherwise known as execution pathway. This pathway is initiated by the cleavage of caspase-
3 and results in DNA fragmentation, degradation of cytoskeletal and nuclear proteins, cross-
linking of proteins, formation of apoptotic bodies, expression of ligands for phagocytic cell
receptors and finally uptake by phagocytic cells (Elmore 2007). The granzyme A pathway
activates a parallel, caspase-independent cell death pathway via single stranded DNA damage
(Martinvalet et al, 2005).
79
Figure 1.18: Intrinsic and extrinsic pathway
80
1.43 Extrinsic Pathway (caspase -8 apoptosis)
The extrinsic signaling pathways that initiate apoptosis involve activation of caspace
3- which is usually activated either by caspase -8 or -9. Activation of caspase -8 involves
transmembrane receptor-mediated interactions which also include death receptors
(FasL/FasR,TNF-α/TNFR1, Apo3L/DR3 (Apo3 ligand/ Death-receptor 3), Apo2L/DR4
(Apo2 ligand/ Death-receptor 4) , and Apo2L/DR5 (Apo2 ligand/ Death-receptor 5) that are
members of the TNF receptor gene super family ( Weber et al 2010: Rubio-Moscardo et al,
2005: Locksley et al, 2001: Suliman et al, 2001: Ashkenazi et al, 1998: Peter and
Kramer,1998: Chicheportiche et al, 1997).
Ashkenazi and Dixit also reported that members of the TNF receptor family share
similar cysteine-rich extracellular domains and have a cytoplasmic domain of about 80 amino
acids called the “death domain” (Ashkenazi and Dixit, 1998). This plays a critical role in
transmitting the death signal from the cell surface to the intracellular signaling pathways. The
sequence of events that define the extrinsic phase of apoptosis are best characterised with the
FasL/ FasR (Fatty acid synthetase ligand /Fatty acid synthetase receptor) and TNF-α /TNFR1
(tumour necrosis factor-alpha /tumour necrosis factor receptor 1) models, which involve
clustering of receptors and binding with the homologous trimeric ligand. Upon ligand
binding, cytoplasmic adapter proteins are recruited which exhibit corresponding death
domains that bind with the receptors.
The binding of Fas ligand to Fas receptor results in the binding of the adapter protein
FADD (Fas-associated death domain) and the binding of TNF ligand to TNF receptor results
in the binding of the adapter protein TRADD (TNF receptor-associated death domain) with
recruitment of FADD and RIP (Receptor-interacting protein) (Wajant, 2002: Hsu et al,
81
1995). FADD then associates with procaspase-8 via dimerization of the death effector
domain, leading to the formation of a mitochondrial permeability transition (MPT).
Subsequently, this causes auto-catalytic activation of procaspase-8 (Pro cysteinyl aspartic
acid-protease 8) (Kischkel et al, 1995). Activation of caspase-8 automatically triggers the
execution phase of apoptosis (Figure 1.18).
1.44 Intrinsic Pathway (mitochondria apoptosis)
Mitochondria apoptosis appears to be much more common than caspase -8 dependent
apoptosis in vivo and this apoptotic pathway is controlled by bcl-2 (B-cell lymphoma protein
2) family of proteins (Cory and Adams, 2002). BH3 protein belonging to bcl-2 protein
family is the only protein that usually regulates the activation of the effectors Bax and Bak
(Figure 1.18). Once Bax and Bak are activated, cytochrome c will be authomatically released
from the mitochondria intermembrane space into the cytosol, where it binds to Apaf-1
inducing its oligomerisation and thereby causing the activation of caspase-9 (Grepsi et al
2010). Some stimuli like, radiation, toxins, hypoxia, hyperthermia, viral infections, free
radicals have been reported to cause such changes in the inner mitochondria leading to an
opening of the MPT pore, loss of the mitochondrial transmembrane potential and release of
two main groups of normally sequestered pro-apoptotic proteins from the intermembrane
space into the cytosol (Saelens et al., 2004). The clustering of procaspase-9 in this manner
leads to caspase-9 activation. Smac/DIABLO and HtrA2/Omi (second mitochondrial
activator of caspases/direct IAP binding protein with low PI) has been reported to promote
apoptosis by inhibiting IAP (inhibitors of apoptosis proteins) activity (Schimmer 2004: Van
Loo et al, 2002).
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The second group of pro-apoptotic proteins, AIF (Apoptosis Inducing Factor),
endonuclease G and CAD (Caspase-Activated DNAse), are released from the mitochondria
during apoptosis, but this is a late event that occurs after the cell has committed to die. AIF
translocates to the nucleus and causes DNA fragmentation into ~50,300 kb pieces and
condensation of peripheral nuclear chromatin (Joza et al, 2001). This early form of nuclear
condensation is referred to as “stage I” condensation (Susin et al, 2000). Endonuclease G also
translocates to the nucleus where it cleaves nuclear chromatin to produce oligonucleosomal
DNA fragments (Li et al, 2001). AIF and endonuclease G both function in a caspase-
independent manner. CAD is subsequently released from the mitochondria and translocates to
the nucleus where, after cleavage by caspase-3, it leads to oligonucleosomal DNA
fragmentation and a more pronounced and advanced chromatin condensation (Enari et al,
1998). This later and more pronounced chromatin condensation is referred to as “stage II”
condensation (Susin et al, 2000).The control and regulation of these apoptotic mitochondrial
events occurs through members of the Bcl-2 family of proteins. The anti-apoptotic members
of the Bcl-2-family appear to block apoptosis by binding either BH3-only proteins or
Bax/Bak (Grepsi et al 2010).
1.45 Perforin/granzyme Pathway
T-cell mediated cytotoxicity is a variant of type IV hypersensitivity where sensitized CD8+
(Cluster of differentiation 8+) cells kill antigen-bearing cells. These cytotoxic T lymphocytes
(CTLs) are able to kill target cells via the extrinsic pathway and the FasL/FasR interaction is
the predominant method of CTL-induced apoptosis (Brunner et al, 2003). Conversely, they
can also exert their cytotoxic effects on tumour cells and virus-infected cells through a new
pathway that involves secretion of the transmembrane pore-forming molecule called perforin
83
with a subsequent exophytic release of cytoplasmic granules through the pore and into the
target cell (Trapani and Smyth, 2002).
The serine proteases granzyme A and granzyme B are the most important component
within the granules. Granzyme B will cleave proteins at aspartate residues and this leads to
activation of procaspase-10 and can cleave factors like ICAD (inhibitor of caspase-activated
DNase) (Sakahira et al, 1998). Barry and Bleackley and others have also shown that
granzyme B can utilise the mitochondrial pathway for amplification of the death signal by
specific cleavage of BID and induction of cytochrome c release (Barry and Bleackley, 2002;
Russell and Ley, 2002). However, granzyme B can also directly activate caspase-3 by passing
the upstream signaling pathways resulting into direct induction of the execution phase of
apoptosis (Elmor, 2007). Goping and co-researchers has suggested that both the
mitochondrial pathway and direct activation of caspase-3 are critical for granzyme B-induced
killing (Goping et al, 2003). Recent research has shown that this method of granzyme B
cytotoxicity is critical as a control mechanism for T-cell expansion of type 2 helper T (Th2)
cells (Devadas et al., 2006). In addition, findings indicate that neither death receptors nor
caspases are involved with the T-cell receptor-induced apoptosis of activated Th2 cells
because blocking their ligands has no effect on apoptosis. On the other hand, Fas-Fas ligand
interaction, adapter proteins with death domains and caspases are all involved in the
apoptosis and regulation of cytotoxic Type 1 helper cells whereas granzyme B has no effect
(Elmore 2007).
Granzyme A is also important in cytotoxic T-cell induced apoptosis and activates
caspase-independent pathways. Once in the cell, granzyme A activates DNA nicking via
DNAse NM23-H1, a tumour suppressor gene product (Fan et al, 2003). This DNAse has an
important role in immune surveillance to prevent cancer through the induction of tumour-cell
84
apoptosis. Granzyme A protease cleaves SET (the nucleosome assembly protein that
normally inhibits the NM23-H1 gene) complex thereby releasing inhibition of NM23-H1,
resulting in apoptotic DNA degradation. In addition to inhibiting NM23-H1, the SET
complex has important functions in chromatin structure and DNA repair. The proteins that
make up this complex (SET, Ape1, pp32, and HMG2) appear to work together to protect
chromatin and DNA structure (Lieberman and Fan, 2003). Therefore, inactivation of this
complex by granzyme A most likely also contributes to apoptosis by blocking the
maintenance of DNA and chromatin structure integrity.
1.46 Execution Pathway
Execution pathway is the final pathway of apoptosis and both extrinsic and intrinsic
pathways end at the point. This phase of apoptosis is initiated by the activation of the
execution caspases. Execution caspases activate cytoplasmic endonuclease, which degrades
nuclear material, and proteases that degrade the nuclear and cytoskeletal proteins. Caspase-
3,caspase-6, and caspase-7 function as effector or “executioner” caspases, cleaving various
substrates including cytokeratins, PARP (Poly (ADP-ribose) polymerase), the plasma
membrane cytoskeletal protein alpha fodrin, the nuclear protein NuMA (Nuclear mitotic
apparatus protein) etc., that ultimately cause the morphological and biochemical changes seen
in apoptotic cells (Slee et al, 2001).
Caspase-3 is known to be the most important of the executioner caspases and is
activated by any of the initiator caspases (caspase-8, caspase-9, or caspase-10). Caspase-3
specifically activates the endonuclease CAD. In proliferating cells CAD is complexed with
its inhibitor, ICAD (Inhibitor of CAD). In apoptotic cells, activated caspase-3 cleaves ICAD
85
to release CAD (Sakahira et al, 1998). CAD then degrades chromosomal DNA within the
nuclei resulting to chromatin condensation. Caspase-3 also triggers cytoskeletal
reorganisation and disintegration of the cell into apoptotic bodies.
Gelsolin, an actin binding protein, has been identified as one of the key substrates of
activated caspase-3. Gelsolin will typically act as a nucleus for actin polymerisation and will
also bind phosphatidyl inositol biphosphate, linking actin organisation and signal
transduction. Caspase-3 will cleave gelsolin and the cleaved fragments of gelsolin, in turn,
cleave actin filaments in a calcium independent manner. These result in disruption of the
cytoskeleton, intracellular transport, cell division, and signal transduction (Kothakota et al,
1997). Phagocytic uptake of apoptotic cells is the last component of apoptosis. Phospholipid
asymmetry and externalization of phosphatidyl serine on the surface of apoptotic cells and
their fragments is the hallmark of this phase. Although the mechanism of phosphatidyl serine
translocation to the outer leaflet of the cell during apoptosis is not well understood, it has
been associated with loss of aminophospholipid translocase activity and nonspecific flip-flop
of phospholipids of various classes (Bratton et al, 1997). Ferraro-Peyret and others have
shown that Fas, caspase-8, and caspase-3 are involved in the regulation of phosphatidyl
serine externalization on oxidatively stressed erythrocytes, however caspase-independent
phosphatidyl serine exposure occurs during apoptosis of primary T lymphocytes (Mandal et
al., 2005: Ferraro-Peyret et al, 2002). The appearance of phosphatidyl serine on the outer
leaflet of apoptotic cells then facilitates non-inflammatory phagocytic recognition, allowing
for their early uptake and disposal (Fadok et al, 2001). This process of early and efficient
uptake with no release of cellular constituents, results in essentially no inflammatory
response.
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1.47 Importance of Apoptosis
Apoptosis plays significant roles in normal physiology relative to its counterpart,
mitosis. Although it demonstrates a complementary but opposite role to mitosis and cell
proliferation in the regulation of various cell populations. It is estimated that to maintain
homeostasis in the adult human body, around 10 billion cells are made each day just to
balance those dying by apoptosis (Renehan et al, 2001). This number can increase
significantly when there is enhanced apoptosis during normal development and aging, or
during disease. Apoptosis is also critically important during various developmental processes
(Opferman and Korsmeyer, 2003: Nijhawan et al, 2000).
Furthermore, apoptosis is significant in getting rid of the body pathogen-invaded
cells; moreover, it is an important component of wound healing due to its involvement in the
removal of inflammatory cells and the evolution of granulation tissue into scar tissue
(Greenhalgh, 1998). Dysregulation of apoptosis during wound healing can lead to pathologic
forms of healing, such as excessive scarring and fibrosis. Apoptosis is also required to
eliminate activated or auto-aggressive immune cells either during maturation in the central
lymphoid organs (bone marrow and thymus) or in peripheral tissues (Osborne, 1996).
Moreover, apoptosis is central to remodelling in the adult, such as the follicular
atresia of the postovulatory follicle and post-weaning mammary gland involution, just to
mention a few (Lund et al, 1996: Tilly, 1991). Further, as organisms’ age, some cells begin to
deteriorate at a faster rate and are eliminated via apoptosis. One theory is that oxidative stress
plays a primary role in the pathophysiology of age-induced apoptosis via accumulated free-
radical damage to mitochondrial DNA (Ozawa, 1995: Harman, 1992). Apoptosis has to be
tightly regulated since excessive or insufficient cell death may lead to pathology, including
cancer.
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1.48 Apoptosis and Necrosis: compare and contrast
Necrosis, a known toxic process whereby the cell is a passive victim and follows an energy-
independent mode of death, has been considered an alternative cell death to apoptosis.
Although necrosis, as a form of cell death, has been a subject of debate since it refers to the
degradative processes that occur after cell death, it is considered by some to be an
inappropriate term to describe the mechanism of cell death (Elmore, 2007). Oncosis is
therefore used to describe a process that leads to necrosis with karyolysis and cell swelling
whereas apoptosis leads to cell death with cell shrinkage, pyknosis, and karyorrhexis (Majno
and Joris, 1995; Levin et al., 1999).
Necrosis is also considered an uncontrolled and passive process that usually affects
large fields of cells whereas apoptosis is controlled and energy-dependent and can affect
individual or clusters of cells. Necrotic cell injury is mediated by two major mechanisms:
interference with the energy supply of the cell; and direct damage to cell membranes.
Whereas, apoptosis is mediated by two major mechanisms: extrinsic or death-receptor
pathway; and the intrinsic or mitochondrial pathway (Figure 1.18). There is also an additional
pathway, known as perforin/granzyme (Elmore, 2007).
Some of the major morphological changes that occur with necrosis include cell
swelling; formation of cytoplasmic vacuoles; distended endoplasmic reticulum; formation of
cytoplasmic blebs; condensed, swollen or ruptured mitochondria; disaggregation and
detachment of ribosomes; disrupted organelle membranes; swollen and ruptured lysosomes;
and eventually disruption of the cell membrane (Trump et al, 1997: Majno and Joris, 1995:
Kerr et al, 1972). This loss of cell-membrane integrity results in the release of the
cytoplasmic contents into the surrounding tissue, sending chemotatic signals with eventual
recruitment of inflammatory cells (Figure 1.19).
88
In contrast to necrotic cells, apoptotic cells do not release their cellular constituents
into the surrounding interstitial tissue and are quickly phagocytosed by macrophages or
adjacent normal cells, and there is ultimately no inflammatory reaction (Kurosaka et al, 2003:
Savill and Fadok, 2000). Although the mechanisms and morphologies of apoptosis and
necrosis differ, there is overlap between these two processes. Research has shown that
necrosis and apoptosis represent morphologic expressions of a shared biochemical network
described as the “apoptosis necrosis continuum” (Zeiss, 2003). For example, two factors that
will convert an ongoing apoptotic process into a necrotic process include a decrease in the
availability of caspases and intracellular ATP (Denecker et al, 2001: Leist et al, 1997).
Whether a cell dies by necrosis or apoptosis depends in part on the nature of the cell death
signal, the tissue type, the developmental stage of the tissue and the physiologic milieu
(Zeiss, 2003: Fiers et al, 1999).
Therefore, distinguishing necrosis from apoptosis is regarded as a difficult task;
especially with the use of conventional histology. This is because the two processes can occur
simultaneously, depending on factors such as the intensity and duration of the stimulus, the
extent of ATP depletion and the availability of caspases (Zeiss, 2003). It is also important to
note that pyknosis and karyorrhexis are not exclusive to apoptosis and can be a part of the
spectrum of cytomorphological changes that occurs with necrosis (Cotran et al, 1999).
89
Apoptosis Vs Necrosis
Figure 1.19: Differences between apoptosis and necrosis
90
1.49 Apoptosis and Cancer
Abnormalities in cell death regulation can be a significant component of diseases such
as cancer. Cancer formation is a possibility when there is dysfunctional regulation of the
normal mechanisms of cell cycle, with either an over proliferation of cells and/or decreased
removal of cells (King and Cidlowski, 1998). In fact, suppression of apoptosis during
carcinogenesis is thought to play a central role in the development and progression of some
cancers (Wong 2011: Kerr et al, 1994). There are a variety of molecular mechanisms that
tumour cells use to suppress apoptosis and some of these molecular mechanisms are briefly
discussed below: Tumour cells can acquire resistance to apoptosis by the expression of anti-
apoptotic proteins such as Bcl-2 (B-cell lymphoma protein 2) or by the down-regulation or
mutation of pro-apoptotic proteins such as Bax (Bcl-2 associated X protein). The expression
of both bcl-2 and bax is regulated by the p53 tumour suppressor gene (Miyashita, 1994).
Vaux and co workers reported that certain forms of human B-cell lymphoma have
overexpression of Bcl-2, and this is one of the first and strongest lines of evidence that failure
of cell death contributes to cancer (Vaux et al, 1988).
Another method of apoptosis suppression in cancer involves evasion of immune
surveillance (Smyth et al, 2001). Certain immune cells (T cells and natural killer cells)
normally destroy tumour cells via the perforin/granzyme B pathway or the death-receptor
pathway. In order to evade immune destruction, some tumour cells will diminish the response
of the death-receptor pathway to FasL produced by T cells. This has been proven to occur in
a variety of ways including down-regulation of the Fas receptor on tumour cells. Other
mechanisms include expression of non-functioning Fas receptor, secretion of high levels of a
soluble form of the Fas receptor that will sequester the Fas ligand or expression of Fas ligand
on the surface of tumour cells (Elnemr et al, 2001: Cheng et al, 1994). In addition, some
91
tumour cells are capable of a Fas ligand-mediated “counter attack” that results in apoptotic
depletion of activated tumour infiltrating lymphocytes (Koyama et al, 2001).
Alterations of various cell signaling pathways can result in dysregulation of apoptosis
and lead to cancer; for example, the p53 tumour suppressor gene is a transcription factor that
regulates the cell cycle. This is the most widely mutated gene in human tumourigenesis
(Wang and Harris, 1997). The critical role of p53 is evident by the fact that it is mutated in
over 50% of all human cancers. p53 can activate DNA repair proteins when DNA has
sustained damage, can hold the cell cycle at the G1/S regulation point on DNA damage
recognition, and can initiate apoptosis if the DNA damage proves to be irreparable
(Pientenpol and Stewart, 2002) and dysregulation of this system can lead to tumourigenesis.
For example, if the p53 gene is damaged (by chemical, radiation, viruses etc), tumour
suppression is severely reduced or people who inherit only one functional copy of this gene
will most likely develop Li–Fraumeni syndrome. This is characterised by the development of
tumours in early adulthood (Gu et al, 2001: Varley et al, 1997).
Other cell signaling pathways that can also be involved in tumour development
include, phosphatidyl inositol 3-kinase/AKT pathway. Up-regulation of the phosphatidyl
inositol 3-kinase/AKT pathway in tumour cells renders them independent of survival signals.
In addition to regulation of apoptosis, this pathway regulates other cellular processes, such as
proliferation, growth, and cytoskeletal rearrangement (Vivanco and Sawyers, 2002).
1.50 GAG’s and apoptosis
GAGs have been shown to play a modulatory role in the apoptotic processes. For
example, heparin has been shown to inhibit glomerular cell apoptosis in cell culture and
92
attenuates trophoblast apoptosis (Bose et al 2005: Ishikawa and Kitamura 1999). The GAG
hyaluronan attenuates apoptosis induced by dexamethasone in malignant multiple myeloma
cells (Vincent et al 2003). Similarly, chondroitin CS and HS have also been reported to have
attenuated apoptosis in fetal lung fibroblasts (Cartel and Post 2005).
However, numerous data indicate the ability of GAGs to induce apoptosis. Hence,
they may contribute to the natural processes of the body for the removal of tumour cells.
Heparin in particular has been shown to induce apoptosis in human hepatoma cells (Karti et
al 2003), human nasopharyngeal carcinoma cells (Li et al 2001) and peripheral blood
neutrophils (Manaster et al 1996), possibly by interfering with transcription factor function
(Berry et al 2004). Likewise, derivatives of heparin and CS also induce apoptosis of
myeloma and breast cancer cells in vitro (Pumphrey et al 2002).
1.51 Overall aims of this study
Comprehensive surveys of previous research into different classes of invertebrates,
including molluscs, have demonstrated that GAG-like compounds, such as HS and/or
heparin-like compounds, and CS and or DS, are present in many species (Medeiros et al,
2000). However, commercial available preparations of GAGs compounds are mainly sourced
from porcine and bovine intestinal or bovine lung tissue. A link between bovine spongiform
encephalopathy and the similar prion-based Creutzfeldt-Jakob disease in humans
(Schonberger, 1998), has limited the use of bovine GAGs in the clinic. Moreover, porcine
GAGs also have problems associated with religious restrictions on its use (Volpi, 2005).
Non-animal sources of GAGs with clinical useful activities are unavailable currently for
pharmaceutical purposes. However, there is scant information on isolation/charactertisation
of GAGs from molluscs such as whelk and cockles. There is even less information on the
93
potential biological activities of these mollusc derived polysaccharides and their potential use
as new therapeutics for the treatment of human disease such as cancer.
The primary aim of the work presented in this thesis is to isolate GAGs from whelks
and cockles using a method similar to that described by Kim et al (1996), albeit with some
slight modifications. Initial pilot studies revealed that novel GAG chains isolated from these
two molluscs contain HS and CS/DS GAGs. The anticancer activities of these mullusc
derived GAGs was assessed and commercial HS and CS/DS, from bovine sources, were used
as comparative controls.
The second aim of this project was to investigate the relationship between the
structure of these mollusc derived GAGs and the observed anticancer activities. Studies have
previously shown that modulation of HS GAGs structure on the surface of tumour cells could
inhibit or promote tumour growth and metastasis (Liu et al, 2002). Understanding the fine
structure and specific biological roles of GAGs has resulted in novel therapeutic approaches,
including the development of HS/heparin-like compounds, which may act as inhibitors of
tumour metastasis (Afratis et al, 2012). The anticancer activities of these HS/heparin related
compounds have been shown to result primarily from their interaction, and inhibitory effects,
on hundreds of different proteins, including FGFs, VEGF etc. The direct inhibition of tumour
cell growth seen with our mollusc derived GAGs indicates a totally new mechanism for GAG
related anticancer activity and the structural difference seen in these polysaccharides must be
determind as a priority.
The third aim of the presented work was to study the possible mechanism of action of
the novel GAGs on cancer cells using cell cycle analysis and determination of apoptotic
induction and to hopefully link with the GAG structural findings.
94
Overall the results obtained from this study will undoubtedly serve as the basis for the future
development of these novel mollusc derived GAGs as potential anticancer agents.
95
Section 2
Experimental Materials and Methods
96
2.0 Experimental materials
PD-10 pre-packed columns were purchased from Amersham Pharmacia Biotech. The
TSK3000PW gel-filtration column and Pro-Pac PA-1 SAX-HPLC column (4.6 x 25cm) was
purchased from Phenomenex (Macclesfield, UK)
Cockles and whelks were purchased from Arndale fish market, Manchester, UK. Polcine HS
and CS commercial GAGs were purchased from Celsus laboratories (Cincinnati, OH, USA).
Heparin sodium salt was purchased from Sigma Aldrich, UK. ). Heparinase I
(Flavobacterium heparinum; EC 4.2.2.7), heparinase II (F. heparinum; no EC number
assigned) and heparinase III (F. heparinum; EC 4.2.2.8) were purchased from Grampian
Enzymes (Orkney, UK).
TEMED, Acrylamide/bisacrylamide 19:1 ratio, 40% solution, Ammonium
persulphate, Cetylpiridium chloride, Ethylene diamineteracetic acid, chondroitinase-ABC
from Proteus Vulgaris (0.83 units/mg), 99% Glycerol, Trizma base (Tris HCl), Cisplatinum
(cis-Diammineplatinum(11)dichloride), 2-(4,5-Dimethylthiazol-2-yl)-2,5-diphenyltetrazolium
bromide (MTT), Acrylamide/bisacrylamide 19 :1 ratio, 40% solution, Foetal calf serum
(FCS) – Biosera, Streptomycin and Penicillin, L-Glutamine, RPMI 1640 (Roswell Park
Memorial Institute) – Biosera, DEAE-Sephacel, Propiodide (PI), (4',6-diamidino-2-
phenylindole (DAPI), Protease from Streptomyces griseus (Type XIV, ≥3.5 units/mg) and
AZURE A dye were purchased from Sigma, UK. Acetone, Ethanol, eppendof tubes,
Micropipettes (10-1000 µl), Micropipettes (10-1000 µl) and other cell culture
laboratory consumables were purchased from Fischer Scientific, UK. Dialysis tubing
‘Visking’ was purchased from iBOTZ, USA. Sodium Chloride, Potassium acetate, Sodium
bicarbonate, Trichloroacetic acid (TCA) and Sulphuric acid were purchased from Merck
Millipore, UK. Bromophenol red and Glyceine (aminoacetic acid) were purchased from
97
Chemicals VWR BDH, UK. Anexin V-FITC stain was purchased from BIORAD, UK.
Phosphate buffer saline was purchased from Partec.
98
2.1 Methods
2.2 Preparation of GAGs
Whelk (Buccinum undatum) and cockle (Cerastoderma edule) from the Irish Sea were
sourced from local fish markets in Fleetwood, UK and were defatted using three 24h
extractions with acetone and dried. The fat-free dried cockles and whelks were crushed into a
fine powder using an industrial blender. Approximately 40g of dried, defatted, pulverised
powder was suspended in 400ml of 0.05 M sodium carbonate buffer (pH 9.2) and 20ml of the
proteolytic enzyme Alcalase (Type XIV, ≥3.5 units/mg; 10 mg/ml) was added to the
suspension in order to detach the carbohydrate chains from proteins. The suspension was
shaken for 48 h at 200 rpm at 60 °C. The digestion mixture was cooled to 4 °C, and
trichloroacetic acid added to a final concentration of 5% (to remove non degraded
proteins/peptides and nucleic acids).
The sample was mixed, allowed to stand for 10 min, and then centrifuged for 20 min
at 8000 rpm. The supernatant was recovered by decanting and the precipitate discarded. 3
volumes of 5% potassium acetate in ethanol were added to one volume of supernatant. After
mixing, the suspension was stored overnight at 4 °C and then centrifuged for 30 min at 8,000
rpm. The supernatant was discarded, and the precipitate was washed with absolute alcohol.
The precipitate was dissolved in 400 ml of 0.2 M NaCl, centrifuged for 30 min at 8,000 rpm
and the insoluble material discarded. GAGs were recovered from the supernatant by addition
of 5 ml of a 5 % solution of cetylpyridinium chloride and the precipitate collected by
centrifugation.
The precipitate was dissolved in 100 ml of 2.5 M NaCl followed by the addition of 5 volumes
of ethanol and the precipitate removed by centrifugation for 30 min at 10,000 rpm. The crude
GAG precipitate was then dissolved in distilled water and dialysed as described below.
99
2.3 Desalting of crude GAGs
Crude GAGs obtained from the extraction procedure were desalted using dialysis
tubing pre- treated with 100mM EDTA. The dialysis tubes containing GAG extracts were
dialysed against 100 volumes of distilled water for 72 hours under constant agitation with the
distilled water changed at 24 hour intervals. After 72 hours, the desalted GAG extracts were
freeze dried and stored at -20 0C for further use.
2.4 Purification of crude GAGs by anion-exchange chromatography
GAG samples (10mg) derived from the shellfish samples were dissolved in 10ml
distilled water and manually injected onto a column (1.5x 5cm) of DEAE-sephacel
equilibrated with 50 mM sodium phosphate buffer, pH 7.0. The column was eluted using a
linear gradient of 0-3 M NaCl in 50mM phosphate buffer, pH 7.0 over a hundred minutes at
flow rate of 1ml/min. The elution was monitored spectrophotometrically at 210, 232 and
254nm and 1ml fractions collected. Peak were pooled, freeze dried and finally desalted using
PD 10 column
2.5 Desalting of purified GAGs fractions
The purified GAGs fractions were desalted on PD-10 column pre-calibrated with
1mg/ml dextran (blue colour) and potassium dichromate (yellow colour) solution (the blue
eluents were equivalent to GAGs, while the yellow eluents were equivalent to salt). The
calibrated column was equilibrated with distilled water; the void volume and salt fractions
were discarded while the GAGs fractions were pooled and stored at -200C overnight before
100
being transferred to the freeze drier. The desalted GAGs samples were lyophilised and a dried
and a pure white, fluffy GAG powder were obtained.
2.6 Enzyme digestion of GAGs
Samples of GAGs (1mg/ml) were treated with either heparinases or chondroitinase
ABC lyase (30mIU) and incubated for 24 hours at 370C.
2.7 Chemical treatment (nitrous acid treatment)
Samples of GAGs were treated with nitrous acid according to the method described by Zhang
et al., 2009. Powdered GAGs (100μg) were dissolved in distilled water (30μl) and 0.5M
sulphuric acid (10 μl) and sodium nitrite (600μg) added. The combined reagents released
gaseous nitrogen and formed nitrous acid. The reaction was halted after 15 minutes by adding
an equal amount of 0.1M NaOH to neutralize excess nitrous acid. Treated samples were used
for PAGE analysis, as described below.
2.8 Polyacrylamide gel electrophoresis (PAGE analysis)
PAGE was conducted on Bio-Rad MiniProtean II systems. A resolving gel (15 ml of 40%
acrylamide, 5 ml of 1.5 M Tris/HCl pH 8.5, 100 μl of APS, 60 μl of TEMED) were poured
vertically, using a gel-pouring stand (Hoffer), between glass plates (16 cm x 32 cm) separated
by 1.5 mm spacers. Butanol saturated with water (0.5 ml) was layered across the top of the
gel and polymerisation, which began at the top of the gel, was completed within 20 min. The
polymerised gel top layer was rinsed thoroughly with water to remove any excess gel and
saturated butanol. Excess water was removed by filter paper.
101
The stacking gel (3 ml of 40% acrylamide, 5 ml of 0.5 M Tris/HCl pH 8.5, 100 μl of
ammonium per sulphate (APS), 60 μl of TEMED and 12 ml of distilled water) was layered
on top of the polymerised gel and a well comb was inserted. Samples were mixed with equal
volume of loading buffer (20% glycerol) and applied to the wells using a micro syringe; a
marker (20% v/v bromophenol blue) was applied to one of the wells. The gel was run at a
constant voltage (200V) in a running buffer (25 mM Tris, 0.192 M glycine pH 8.3) until the
tracking dye in the marker lane, reached the bottom of the gel. Gels were stained with
aqueous 0.5 %Azure A under constant agitation for about 2 minutes and were destained by
successive washes with distilled water and gels were scanned to preserve gels images.
2.9 Superose-12 size exclusion chromatography
Samples (at 10mg/ml) in a total volume of 20ul of water were applied to a Sepharose-
12 column, eluted in 0.2M ammonium hydrogen carbonate at a flow rate of 0.5ml/minute and
0.5ml fractions collcted. Column Vo and Vt values were established by application of
Bromophenol blue and sodium dichromate (1mg/ml).
Vo fraction 15/16
Vt fraction 34/35
Fractions were assessed for GAG content by cellulose acetate dot blotting.
102
2.10 Cellulose acetate dot blotting of GAGs
Cellulose acetate sheets were marked with a grid of 1cm2 squares using a pencil. Multiple
applications of each fraction were applied to the membrane using a pipette. The acetate sheet
was dried thoroughly between applications in an oven at 750C for 5 minutes each. Following
the final drying the sheet was stained using a solution of 0.5% Azure A stain for 10-20
seconds, then de-stained in tap water until a good contrast between stained dots and
background was achieved.
2.11 Gel-filtration (TSK G2000 SW column)
The TSK column was equilibrated in normal saline overnight prior the experiment. 20 µl of
the filtered oligosaccharides obtained from each heparinase enzyme samples (shell fish and
commercial HS/ Heparin) were injected via 20µl sample loop into the equilibrated column at
a flow rate 250 µl/ml for 180 minutes and the elutes were monitored at 232 nm.
2.12 Disaccharide analysis of GAG chain by strong anion-exchange high
Performance liquid chromatography (SAX-HPLC)
Samples from enzymes digestion assay were applied to a Pro-Pac PA-1 SAX-HPLC
column (4.6 x 25cm) pre-equilibrated in water adjusted to pH 3.5 with HCl at a flow rate 1
ml/min. The disaccharides were resolved using a linear gradient of 0 -3M NaCl in deionised
water, pH 3.5 for 70 min at flow rate of 1ml/min. Elutes were monitored for UV absorbance
at 232nm and peaks were identified according to standard derived from commercial CS/DS
and HS.
103
2.13 Determination of cells viability (MTT assay).
The breast cancer cell MDA468 and MDANQ01, and human lymphoblastic and
erythrocytic cell line (Molt-4 and K562) were grown in RPMI 1640 medium supplemented
with 1 % L-glutamine, 1 % of 100 Units/ml penicillin and 0.1 mg/ml streptomycin and 10%
inactivated FCS. While the ovarian cell line HeLa and fibroblast cell line 3T3 were grown in
DMEM medium supplemented with 20 % inactivated FCS, 1 % L- glutamine, 1 % of 100
units/ml penicillin & 0.1 mg/ml streptomycin. All cell lines were maintained in a humidified
incubator with an atmosphere of 95% air and 5% CO2 at 37°C.
Cell viability was determined by the MTT
(3-(4,5dimethylthiazol2-yl)-2,5 diphenyltetrazolium bromide) test method. Cells were
cultured overnight in 96-well plates (2.0 x 10 4 cells/ well) containing 100 µl medium prior to
treatment with crude GAG extract, commercial GAGs and cisplatinum at 37°C. A pilot study
was conducted to choose the dose range used for this experiment. This was followed by
addition of 100 µl of fresh medium containing various concentrations of GAGs (10-100
µg/ml) or cisplatinum (0.35-25mM/ml) into each well, and incubated for another 96 hrs. The
metabolic activity of each well was determined by the (MTT) assay and compared to those of
untreated cells. At the end of the incubation period, 50µl of MTT solution (5 mg/ml in PBS)
was added to each well and incubated for three hours at 370C. After incubation the
supernatants were carefully aspirated, then 200 μl of DMSO was added to each well and the
plates agitated to dissolve the crystal product. Cell viability was determined based on
mitochondrial conversion of 3[4,5-dimethylthiazol-2-yl] 2,5-diphenyltetrazolium bromide
(MTT) to formazan. The amount of MTT converted to formazan is indicative of the number
of viable cells.
104
The plates were gently agitated until the colour reaction was uniform and the
absorbance was measured at 570 nm using a multi-well plate reader, Sigma Plot 2000
software was used for data analysis. The cell viability effects from exposure of cells to each
concentration of crude whelk GAGs, commercial GAGs and cisplatinum were analysed as
percentages of the control cell absorbance, which were obtained from control wells plated
in RPMI,1% L- glutamate and 10% FCS media. The average cell survival obtained from
triplicate determinations at each concentration was plotted as a dose response curve. The 50%
inhibition concentration (IC50) of the active substances was determined as the lowest
concentration which reduced cell growth by 50 % in treated compared to untreated cells.
2.14 Flow Cytometry Analyses of DNA Content (Cell cycle analysis).
Cells were seeded into 25-cm plastic sterile culture flasks, and incubated for 24 hours
prior to treatment with different concentrations of crude and purified GAGs samples. Cells
were harvested at different time intervals (8-48 hours), centrifuged at 1500 rpm for 5 minutes,
washed three times with phosphate buffer saline (PBS) and fixed in ice cold 70% (v/v)
ethanol for 30 minutes. Before analysis, cells were centrifuged to remove ethanol and washed
with PBS three times. Cells were then incubated at room temperature with 50 µl of
Ribonuclease A (RNase) (50mg/ml) and finally stained with a solution containing 50 g/ml
propidium iodide (PI) for 30 min in the dark. The stained samples were analysed with Partec
flow cytometer. The cell cycle distribution was evaluated on DNA plots by Partec cyflow
space version 2.4 software.
105
2.15 Annexin V-FITC apoptosis detection
Cells were seeded into sterile 6 well plates at 5 x 105 cells/ml, and incubated with or
without GAG extracts at 370C. Cells were harvested at different time intervals (8-48 hours),
centrifuged at 1500 rpm for 5 minutes, washed twice with cold PBS and resuspended in 1x
binding buffer (0.1M HEPES, 1.4 M NaCl and 25 mM CaCl2) at a concentration of 1 x 106
cells/ml. Cells (100 µl) were transferred into 5 ml culture tubes and stained with Annexin V
FITC (5 µl) and PI (10 µl). The stained cells were gently vortexed and then incubated in the
dark for 15 minutes at room temperature. 400 µl of 1 x binding buffer was added to each tube
prior to analysis using a BD flow cytometer.
2.16 DAPI fluorescent microscopy for apoptosis detection
Cells were seeded into sterile 8 well plates at 5 x 105 cells/ml, and incubated with or
without GAG samples at 370C. Cells were harvested at different time intervals (8-48 hours).
The harvested cells were washed twice with cold PBS followed by 1x binding buffer (0.1M
HEPES, 1.4 M NaCl and 25 mM CaCl2). The cells were immediately stained with DAPI and
incubated in the dark for 10 minutes before finally being rinsed with binding buffer. The
stained cells were viewed under the highest lens objective and the images obtained were
scanned by Hamatsu 1394 ORCA-285 camera.
106
2.17 Statistical analysis
All of the results represent the mean ± SEM from triplicate experiments performed in
a parallel manner unless otherwise indicated. Statistical comparisons between groups were
made using one-way ANOVA followed by Student’s t-test, and significant differences were
indicated as p<0.05 and highly significant as p<0.01
107
SECTION 3
RESULTS
108
3.0 Biological evaluation of cockle derived GAG mixtures
3.1 Effects of cockle derived GAG mixtures on MDA468 breast cancer cell growth
(MTT assay results)
The effects of crude cockle GAG mixtures on MDA468 breast cancer cell
proliferation were measured using the MTT assay. Cells were exposed to different
concentrations of crude cockle GAGs (10-100 μg/ml) for 96 hours. Crude cockle GAG
treatment had no growth inhibitory effect on the cell proliferation of MDA468 cell line
(Figure.3.1A). Other commercial sourced GAGs (HS and CS) derived from bovine sources
were tested along with crude cockle GAG on this cell line and none demonsrated any growth
inhibitory effect on MDA468 breast cancer cell, as illustrated in Figure 3.1B. However,
cisplatin, a standard anticancer drug did show growth inhibitory effects on MDA468 cell
proliferation and this serve as a positive growth inhibitory control for all subsequent MTT
experiments (Figure 3.1B).
109
A
0
0.2
0.4
0.6
0.8
1
1.2
1.4
1.6
0 0.39 0.78 1.56 3.12 6.25 12.5 25
Abso
rban
ce af
ter 9
6 hou
rs inc
ubat
ion
Concentrations in µM/ml
Antiproliferative effect of cisplatin on MDA468 breast cancer cell line
Cisplatin
0
0.2
0.4
0.6
0.8
1
1.2
1.4
1.6
0 10 20 30 50 60 80 100
Abso
rban
ce af
ter 9
6 hou
rs inc
ubat
ion
Concentrations in µg/ml
Proliferative effect of cockle GAG on MDA468 breast
cancer cell line
Cockle GAG
B
0
0.2
0.4
0.6
0.8
1
1.2
1.4
1.6
0 10 20 30 50 60 80 100
Absor
bance
after
96 ho
urs in
cubati
on
Concentrations in µg/ml
Proliferative effects of GAGs on MDA468 breast cancer cell line
HS
CS
Cockle
Figure 3.1: MTT cell viability assay for MDA468 cells after treatment with cockle
derived and commercially sourced GAG chains.
Cells were incubated with various concentrations of GAGs for 96 hours after which time cell viability was
measured using an MTT assay (A) Cockle GAGs and cisplatin as a positive inhibitory control, (B) Commercial
and cockle GAGs with cisplatin as a positive control. Each value is presented as the mean SEM of three
independent determinations. The bars in each chart are presented as relative values in comparison to untreated
cells.
Abbreviations: *-Significant (p≤0.05): **-Highly significant (p≤0.01)
** *
110
3.2 Effects of Cockle derived GAG mixtures on the MDANQ01 breast cancer cell
In order to further examine any possible anti-cancer activity of cockle derived GAGs
may have on breast cancer, the crude cockle GAG extracts was also exposed to another breast
cancer cell (MDANQ01) using the MTT assay. Similarly, the crude cockle GAG did not
show any growth inhibitory effect on MDANQ01 breast cancer cell proliferation (Figure
3.2A). Moreover, MDANQ01 cells treated with the commercial GAGs (HS and CS) also
showed no growth inhibitory effect (Figure 3.2B). However, cisplatin standard anti-cancer
drug did exhibits growth inhibitory effects on MDANQ01 cell after the same period of
exposure to the crude extract (Figure 3.2A and B).
111
A
0
0.2
0.4
0.6
0.8
1
1.2
1.4
1.6
0 0.39 0.78 1.56 3.12 6.25 12.5 25
Abso
rban
ce af
ter 9
6 ho
urs i
ncub
atio
n
Concentration in µM/ml
Antiproliferative effect of cisplatin on MDANQ01 breast cancer celll line
Cisplatin
0
0.2
0.4
0.6
0.8
1
1.2
1.4
1.6
0 10 20 30 50 60 80 100
Abso
rban
ce af
ter 9
6 ho
urs i
ncub
atio
nConcentrations in µg/ml
Proliferative effect of cockle GAG on MDANQ01 breast
cancer cell line
Cockle GAG
B
0
0.2
0.4
0.6
0.8
1
1.2
1.4
1.6
0 10 20 30 50 60 80 100
Abso
rtban
ce aft
er 96
hours
incu
batio
n
Concentrations in µg/ml
Proliferative effects of GAGs on MDANQ01 breast cancer cell line
HS
CS
Cockle
Figure 3.2: MTT cell viability assay for MDANQ01 cells after treatment with cockle
derived and commercially sourced GAG chains.
Cells were incubated with various concentrations of GAGs for 96 hours after which time cell viability was
measured using an MTT assay (A) Cockle GAGs and cisplatin as a positive inhibitory control, (B) Commercial
and cockle GAGs with cisplatin as a positive control. Each value is presented as the mean SEM of three
independent determinations. The bars in each chart are presented as relative values in comparison to untreated
cells.Abbreviations: *-Significant (p≤0.05): **-Highly significant (p≤0.01)
**
*
*
112
3.3 Effect of crude cockle GAG mixture on human lymphoblastic leukaemia
(MOLT-4) cell proliferation in vitro
Despite the lack of anticancer activity seen with the breast cancer cell lines, the crude
cockle GAGs was also tested on other cancer cell lines. The effects of crude cockle GAGs on
cancer cell proliferation using a lymphoblastic leukaemia cell line (MOLT-4) showed much
more promise. This cell line was similarly exposed to different concentrations of crude cockle
GAGs (10-100 μg/ml) for 96 hours using an MTT assay.
Crude cockle GAGs decreased significantly the proliferation of MOLT-4 cell
(p<0.001) in a dose dependent manner with a recorded IC50 of 16µg/ml (Figure 3.3A).
According to the standard criteria set by the National Cancer Institute (Chen et al, 1988;
Geran et al, 1972), crude extracts having IC50 values of less than 20 µg/ml are considered
active against the tested cancer cell lines and this recommendation categorised this crude
extract as a potential anti-leukaemia drug.
The ability of the crude extract to inhibit cell proliferation of leukaemia cell lines was
also compared favourably with the anti-proliferative effect of the DNA damaged anti-cancer
drug (cisplatinum) (Figure 3.3A). These results show the potential of cockle derived GAGs as
a future anti-leukaemia drug.
Almost as interesting as the anticancer activity of the cockle derived GAG was the
complete lack of anticancer activity with the commercial GAGs (HS and CS) on the MOLT-4
cell line
(Figure 3.3B). These results suggest for the first time that GAGs chains may have selective
anticancer activity against some cancer cell lines and that this based on their animal origin
and ultimately their fine structure.
113
A
0
0.2
0.4
0.6
0.8
1
1.2
1.4
0 0.39 0.78 1.56 3.12 6.25 12.5 25
Abso
rbanc
e afte
r 96 h
ours
incub
ation
Concentrations in µM/ml
Antiproliferative effect of cisplatin on MOLT-4
Leukemia cell line
Cisplatin
0
0.2
0.4
0.6
0.8
1
1.2
1.4
0 10 20 30 50 60 80 100
Abso
rbanc
e afte
r 96 h
ours
incub
ation
Concentrations in µg/ml
Antiproliferative effect of cockle GAGs on MOLT-4
Leukemia cell line
Cockle GAGs
B
Figure 3.3: MTT cell viability assay for MOLT-4 lymphoblastic leukaemia cells after
treatment with cockle derived and commercially sourced GAG chains.
Cells were incubated with various concentrations of GAGs for 96 hours after which time cell viability was
measured using an MTT assay (A) Cockle GAGs and Cisplatin as a positive inhibitory control (B) Commercial
GAGs and Cisplatin as a positive control. Each value is presented as the mean SEM of three independent
determinations. The bars in each chart are presented as relative values in comparison to untreated cells.
Abbreviations: *-Significant (p≤0.05) **-Highly significant (p≤0.01).
**
**
*
114
3.4 Effects of crude cockle GAG extracts on the growth of K562 erythroleukaemia
cells in vitro.
In order to investigate fully the selective activity of crude cockle GAGs against some
cancer cells, its effects on cell proliferation of erythroleukaemia cell line (K562) was also
measured using MTT assay. Crude cockle GAGs were shown to decrease proliferation of
K562 cells in a dose –dependent manner with a recorded IC50 of 52 µg/ml [Figure 3.4 (A)].
Similarly, the growth inhibitory activity of the cockle GAG extract on K562 leukaemia cell
line was also comparable to the growth inhibitory effect of the DNA damaged anti-cancer
drug (cisplatin) (Figure3.4A). These results suggest that the cockle GAG extract has
comparative activity with the standard anti-cancer drug (cisplatin) to treat this leukaemia cell
line. Again all commercial GAGs (HS and CS) tested along with the crude extract showed no
inhibitory effect on K562 cell proliferation (Figure 3.4B).
115
A
B
Figure 3.4: Concentration-dependent effect of Cockle GAG extracts on K562
erythroleukaemia cell viability.
Cells were incubated with various concentrations of cockle GAGs extracts for 96 hours after which time cell
viability was measured using an MTT assay (A) cockle GAGs and Cisplatin as a positive inhibitory control, (B)
commercial and cockle GAGs with cisplatin as a positive control. Each value is presented as the mean SEM of
three independent determinations. The bars in each chart are presented as relative values in comparison to
untreated cells.
Abbreviations: *-Significant (p≤0.05): **-Highly significant (p≤0.01).
**
*
*
*
*
**
116
3.5 Effect of cockle GAG mixtures on 3T3 normal fibroblast cell line
The cockle derived GAGs have demonstrated a degree of selective activity against
some cancer cells in vitro. Selectivity is one of the positive characteristics of any potent anti-
cancer drug for future development. For this to be fully established, selective activity of crude
cockle GAGs extracts was tested on the standard, non cancerous, 3T3-fibroblast cell line.
Interestingly, the crude extract did not show any growth inhibitory effect on the 3T3 cells as
shown in Figure 3.5. This result suggests that this extract may be highly selective against the
leukemic cell lines; however this needs to be established with a much wider range of normal
cell type e.g. MCF-12, C13589, MCF-12F and HUVEC.
117
0
0.2
0.4
0.6
0.8
1
1.2
0 10 20 30 50 60 80 100
Abso
rban
ce af
ter 9
6 ho
urs
incu
batio
nn
Concentrations in µg/ml
Proliferative effect of cockle GAG on 3T3 normal fibroblast cell line
Cockle GAG
Figure 3.5: MTT cell viability assay for normal fibroblast (3T3) cells after treatment
with cockle GAGs.
Cells were incubated with various concentrations of cockle GAGs for 96 hours after which time cell viability
was measured using MTT assay and cisplatin was used as a positive inhibitory control. Each value is presented
as the mean SEM of three independent determinations. The bars in each chart are presented as relative values in
comparison to untreated cells.
118
3.6 Cell cycle analysis of the MOLT-4 cell line after treatment with cockle GAG
extracts
Our preliminary studies have highlighted that cockle derived GAGs induces cell death
in leukaemia cell lines including MOLT-4 cell line; However, the mechanism of this
anticancer activity was initially unknown. Therefore, the mechanism of cell death induced by
crude cockle GAGs treatment on leukaemia cell using MOLT-4 cell line was examined by
subjecting treated and untreated cells to cell cycle analysis by flow cytometry. A pilot study
was conducted to choose the dose used for this experiment. Results obtained from this study
demonstrated marked disruptive effects on MOLT-4 DNA composition following a brief (16-
24 hours) treatment with the high concentration (50 µg/ml) of the crude extract [Figure 3.6 (i)
A-C]. The dose was chosen based on the result obtained from pilot study.
Significant MOLT-4 cell cycle arrest at G1phase with crude cockle GAGs was
observed after 16 hours incubations using 50μg/ml with concomitant cell arrest at both G1
and G2/M-phase at 24 hours incubations. 16 hours incubations of the cell with 50μg/ml crude
cockle GAGs increased the G1 phase population by 13 % and 20 % at 24 hours. 24 hours
incubations also increased the cell population at G2/M-phase by 15 %. Crude cockle GAGs
decreased the S- phase population by 13 % at 16 hours and 35 % at 24 hours. The observed
effect of the extract on the cell cycle of MOLT-4 cells were statistically significant (p< 0.05)
at 16 hours and highly significant (p<0.01) at 24 hours; when compared the corresponding
values of the test samples with the control [Figure 3.6 (i) A-C].
119
Cell cycle arrest caused by cockle GAGs treatment on MOLT-4 leukemia cell line
B 16 hours Untreated Treated
Fig.3a (iii)
Untreated Treated
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G1% S% G2M% CV%G1 CV%G2M Mn G2M Mn G1 G2M/G1 ChiSqu.31.25 39.10 29.64 6.75 6.98 83.17 41.41 2.008 3.31
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G1% S% G2M% CV%G1 CV%G2M Mn G2M Mn G1 G2M/G1 ChiSqu.46.27 19.60 34.13 6.15 6.96 80.60 40.20 2.005 3.89
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Fig.3a (iii)
Untreated Treated
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G1% S% G2M% CV%G1 CV%G2M Mn G2M Mn G1 G2M/G1 ChiSqu.31.25 39.10 29.64 6.75 6.98 83.17 41.41 2.008 3.31
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partec PASFile: DorcasMol-4 20ug ck 24h 200313_1 Date: 20-03-2013 Time: 13:04:01 Particles: 0 (of 10890 acquired)
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G1% S% G2M% CV%G1 CV%G2M Mn G2M Mn G1 G2M/G1 ChiSqu.46.27 19.60 34.13 6.15 6.96 80.60 40.20 2.005 3.89
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C 24 hours
Untreated Treated
Fig.3a (iv)
Untreated Treated
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G1% S% G2M% CV%G1 CV%G2M Mn G2M Mn G1 G2M/G1 ChiSqu.41.57 23.44 34.98 5.91 5.92 90.00 46.00 1.957 0.25
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G1% S% G2M% CV%G1 CV%G2M Mn G2M Mn G1 G2M/G1 ChiSqu.48.39 6.14 45.47 10.69 13.62 91.96 47.45 1.938 13.32
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Fig.3a (iv)
Untreated Treated
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G1% S% G2M% CV%G1 CV%G2M Mn G2M Mn G1 G2M/G1 ChiSqu.41.57 23.44 34.98 5.91 5.92 90.00 46.00 1.957 0.25
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G1% S% G2M% CV%G1 CV%G2M Mn G2M Mn G1 G2M/G1 ChiSqu.48.39 6.14 45.47 10.69 13.62 91.96 47.45 1.938 13.32
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G1
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G1
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A
*
*
*
**
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120
Figure 3.6 (i): Cell cycle analysis of MOLT-4 lymphoblastic leukaemia cell line
following treatment with 50µg/ml of cockle GAG extracts.
MOLT-4 cell were stained with PI stain and subjected to cell cycle analysis by flow cytometry. (A) Charts
showed averages of three independent experiments after treatment with or without crude cockle GAGs. (B)
Flow cytometry of MOLT-4 cells after 16 and 24 hours incubation without GAGs. (C) Flow cytometry
histogram of MOLT-4 cells after 16 and 24 hours incubation with 50 µg/ml crude cockle GAGs.
Abbreviations: *-Significant (p≤0.05): **-Highly significant (p≤0.01).
121
To investigate whether the deleterious effect of the crude extract on MOLT-4 cell was
dose-dependent, we also examined its effect on DNA composition of MOLT-4 cell line
following treatment with lower concentration (20µg/ml) of the crude extract, using cell cycle
analysis by flow cytometry. Results obtained showed time-dependent marked disruptive
effects similar to that obtained for the higher concentration (50µg/ml) of the crude extract on
MOLT-4 cell cycle [Figure 3.7 (ii) A-C]. The DNA disruptive effect was assessed between 8
and 48 hours time intervals using lower concentrations (20µg/ml) of the crude extract.
Significant MOLT-4 cell cycle arrest at G1 and G2/M-phase with concomitant cell reduction
at S-phase was also observed at 16 and 24 hours following cockle GAG mixture treatment
(20μg/ml).
Additionally, 16 hours incubations of the cell with 20μg/ml crude cockle GAGs
increased the G1 phase population by 4 % and 21 % at 24 hours. 24 hours incubations also
increased the cell population at G2/M-phase by 6 and 11 % respectively [Figure 3.6 (ii) A-C].
Low concentration of crude cockle GAGs decreased the S- phase population by 10 % at 16
hours and 32 % at 24 hours. The observed effect of the extract on the MOLT-4 cell cycle
were statistically significant (p< 0.05) when comparing the corresponding values of the test
samples with the control. There was no noticeable effect observed at 8 and 48 hours
incubations on both concentrations tested (result not shown).
122
A
Cell cycle arrest caused by cockle treatment on MOLT-4 leukemia cell line
B 16 hours
C 24 hours
Untreated
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G1% S% G2M% CV%G1 CV%G2M Mn G2M Mn G1 G2M/G1 ChiSqu.31.25 39.10 29.64 6.75 6.98 83.17 41.41 2.008 3.31
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G1% S% G2M% CV%G1 CV%G2M Mn G2M Mn G1 G2M/G1 ChiSqu.31.25 39.10 29.64 6.75 6.98 83.17 41.41 2.008 3.31
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G1% S% G2M% CV%G1 CV%G2M Mn G2M Mn G1 G2M/G1 ChiSqu.46.56 19.94 33.50 5.80 6.46 81.42 40.63 2.004 3.76
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G1% S% G2M% CV%G1 CV%G2M Mn G2M Mn G1 G2M/G1 ChiSqu.41.57 23.44 34.98 5.91 5.92 90.00 46.00 1.957 0.25
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G1% S% G2M% CV%G1 CV%G2M Mn G2M Mn G1 G2M/G1 ChiSqu.48.39 6.14 45.47 10.69 13.62 91.96 47.45 1.938 13.32
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123
Figure 3.6 (ii): Cell cycle analysis of MOLT-4 lymphoblastic leukemia cell line following
treatment with low concentration (20µg/ml) of cockle GAG extract.
MOLT-4 cell were stained with PI stain and subjected to cell cycle analysis by flow cytometry (A). Charts
showed averages of three independent experiments after treatment with or without crude cockle GAGs. (B)
Flow cytometry of MOLT-4 cells after 16 hours incubations with or without crude cockle GAGs. (C) Flow
cytometry of MOLT-4 cells after 24 hours incubation with or without crude cockle GAGs.
Abbreviations: *-Significant (p≤0.05): **-Highly significant (p≤0.01)
124
3.7 Annexin V-FITC Apoptosis Assay of the MOLT-4 Lymphoblastic leukemia cell line
following treatment with crude cockle GAG
The role of apoptosis in the anticancer effects seen with the cockle GAG extracts was studied
using the Annexin V apoptotic assay induced by crude cockle GAG on the MOLT-4
leukemia cell line. We incubated different concentrations obtained from a pilot study (20 &
50 µg/ml) of the crude cockle extract with the MOLT-4 cells at different time intervals (8-48
hours). Both treated and untreated cells were stained with both PI and annexin V-FITC stains
and analysed by flow cytometry. The results obtained demonstrate that the numbers of early
apoptotic cells increased significantly at both 16 (p≤0.01) and 24 (p≤0.01) hours time points
following incubation with cockle GAGs when compared with the corresponding values of the
control group. At 16 hours post-treatment, the proportion of early apoptotic cells in the cockle
GAG treated cells reached 4.36%, which was significantly higher (p<0.05) than the control
group (0.68%) [Figure 3.7(A-C)]. At 24 hours post treatment, the proportion of early
apoptotic cells increased from 0.48% (control) to 6.95% (cockle GAG). This finding suggests
that the anticancer effects seen with crude cockle GAGs on the leukaemia cell line is, in part,
linked to time-dependent apoptosis.
However, there was no noticeable apoptotic effect observed at 8 and 48 hours for both
concentrations treated (results not shown).
125
A Apoptosis induced by cockle GAG treatment on MOLT-4 leukemia cell line
B 16 hours
Untreated Treated
C 24 hours Untreated Treated
24 hours 16 hours
**
*
*
**
126
Figure 3.7: Detection of Apoptotic MOLT-4 cells treated with cockle GAG‘s extracts by
Annexin V Staining.
MOLT-4 cells were treated with cockle crude GAGs for 16 and 24 hours and then stained using Annexin V-
FITC and PI provided in the Annexin V-FITC Apoptosis Detection Kit (see materials and methods). The
combination of Annexin V-FITC and PI allows for the distinction between early apoptotic cells (annexin V-
FITC positive), late apoptotic and/or necrotic cells (Annexin V-FITC and PI positive), necrotic (PI stained
positive) and viable cells (unstained). (A) MOLT-4 cell treated with or without cockle GAGs for 16 and 24
hours respectively. (B) MOLT-4 cell treated with or without cockle GAGs for 16 hours. (C) MOLT-4 cells
treated with or without cockle GAGs for 24 hours.
Abbreviations: *-Significant (p≤0.05): **-Highly significant (p≤0.01).
127
Table 1: Summary of biological effects of cockle GAGs
MDA468
breast
cancer
cell line
MDANQ01
breast
cancer cell
line
K562
erythrocytic
leukemia cell
line
MOLT-4
lymphoblastic
leukemia cell
line
3T3
normal
fibroblast
cell line
Proliferative
assay results
Supported
cell
growth
Supported
cell growth
Inhibited cell
growth
Inhibited cell
growth
Supported
cell growth
IC50 - - 52µg/ml 16µg/ml -
Cell cycle
arrest
- - - Induced cell
cycle arrest
at both S and
G2M phase
-
Apoptosis
detection
assay
- - - Induced
early
apoptosis
128
SECTION 3B
Biological assay results for whelk GAG
Mixtures
129
3.8 Effect of crude whelk GAG extracts on the growth of the MDANQ01 breast
cancer cell line
The proliferation of MDANQ01 breast cancer cells was found to be inhibited strongly by
crude whelk GAG extracts with a recorded IC50 of 25.14 µg/ml (Figure 3.8A). The observed
inhibitory effect of whelk GAGs on this cell line compared favourably with cisplatin (a
DNA-damaging agent) anticancer drug (Figure 3.8A-B). The results obtained are in stark
contrast to the activites seen with cockle GAG extracts on this breast cancer cell line. This
may indicate the presence of unique structural differences between the GAG chain present in
the whelk and cockle samples. Again, the commercial GAG samples of HS and CS failed to
show any appreciable anticancer effects (Figure 3.8B). These findings are unique and identify
whelk derived GAG chains as potential treatments for breast cancer. The selective nature of
this activity between whelk and cockle GAGs is also a fascinating new discovery with huge
potential for specific targeted therapy in the treatment of different cancers.
130
A
B
0
0.2
0.4
0.6
0.8
1
1.2
1.4
1.6
0 10 20 30 50 60 80 100
Abso
rban
ce af
ter 9
6 hou
rs inc
ubat
ion
Concentrations in µg/ml
Proliferative effects of commercial GAGs on MDANQ01 breast cancer cell line
HS
CS
Figure 3.8: MTT cell viability assay for MDANQ01 cells after treatment with Whelk
extract and commercial GAGs.
Cells were incubated with various concentrations of GAGs for 96 hours after which time cell viability was
measured using an MTT assay (A) whelk extract GAGs with Cisplatin as a positive inhibitory control, (B)
commercial GAGs with cisplatin as a positive control. Each value is presented as the mean SEM of three
independent determinations. The bars in each chart are presented as relative values in comparison to untreated
cells.
Abbreviations: * Significant (p≤0.05): **-Highly significant (p≤0.01)
**
*
**
131
3.9 Effect of crude whelk GAG extracts on the growth of MDA468 breast cancer
cells
The proliferation of MDA468 breast cancer cell was similarly inhibited, in a dose
dependent, by crude whelk GAGs with a recorded IC50 of 70.94 µg/ml (Figure 3.9A). In
contrast, the whelk GAGs had a more profound anticancer activity with the MDANQ01 cell
line. Again the activity was dose-dependent with an IC50 of 25.14µg/ml (Figure 3.8A). These
results suggest that the MDANQ01 cell line is more sensitive to whelk GAGs treatment than
MDA468 cells. The observed inhibitory effect of whelk GAGs on this cell line also compared
favourably with cisplatin (a DNA-damaging agent) anti-cancer agent at a concentration range
between 1-25 µM with a recorded IC50 of 0.88 µM (Figure 3.9A-B). Once again, the
commercial GAGs (HS and CS) (Figure 3.9B), did not have growth inhibitory effect on this
cell line but rather serve as a growth catalyst for this cell line.
These results suggest that the whelk derived GAG’s possesses a unique activity
against the growth of breast cancer cells and shows great potential for the treatment of this
disease. Indeed the differences in IC50 values for the two breast cancer cell lines suggests that
the whelk derived GAG’s could be selective to certain cell types and this selectivity may well
be important in targeting the effects of these molecules towards tumour cells.
Further studies to establish the effects of these GAG’s on other tumour and normal cell lines
have also been performed; the results of which are outlined in the following section.
132
A
0
0.2
0.4
0.6
0.8
1
1.2
1.4
1.6
0 10 20 30 50 60 80 100
Abso
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rs inc
ubat
ion
Concentrations in µg/ml
Antiproliferative effect of whelk GAG on MDA468 breast cancer cell line
Whelk GAG
0
0.2
0.4
0.6
0.8
1
1.2
1.4
1.6
0 0.39 0.78 1.56 3.12 6.25 12.5 25
Abso
rban
ce af
ter 9
6 hou
rs inc
ubat
ion
Concentrations in µg/ml
Antiproliferative effect of cisplatin on MDA468 cell
line
Cisplatin
B
0
0.2
0.4
0.6
0.8
1
1.2
1.4
1.6
0 10 20 30 50 60 80 100
Abso
rbanc
e afte
r 96 h
ours
incub
ation
Concentrations in µg/ml
Antiproliferative effects of commercial GAGs on MDA468breast cancer cell line
CS
HS
Figure 3.9: Concentration-dependent effect of whelk GAG extracts on MDA468 breast
cancer cell viability.
Cells were incubated with various concentrations of GAGs for 96 hours after which time cell viability was
measured using an MTT assay (A) Whelk crude GAGs with Cisplatin as a positive inhibitory control, (B)
Commercial and crude whelk GAGs with cisplatin as a positive control. Each value is presented as the mean
SEM of three independent determinations. The bars in each chart are presented as relative values in comparison
to untreated cells.
Abreviation: * Significant (p≤0.05): ** Highly significant (p≤0.01)
*
** ** ** **
**
* *
* **
133
3.10 Effect of crude whelk GAG extracts on the growth of K562 and MOLT-4
leukaemia cells lines (K562 and MOLT-4)
Further investigation of anticancer effects of crude whelk GAG was performed using
two different cancer cell lines (MOLT-4 and K562). The results obtained from this study
confirm the whelk derived GAGs anticancer activities. The anti-proliferative activities of
these polysaccharides are dose-dependent on both leukaemia cell lines with the best activity
seen against K562 cell line (Figure 3.10B). Suprisingly, the growth inhibitory activities of the
crude whelk was more pronounced on erythroleukaemia cell line (K562) than MDANQ01
breast cancer cell. The recorded IC50 for crude whelk GAG exctract on k562 leukemia cell
was 14µg/ml. Contrarily, the crude whelk GAG extracts inhibited the growth of MOLT-4
leukaemia cell proliferation in a concentration-dependent manner with arecorded IC50 of
41.11µg/ml and the lowest concentration (10µg/ml) of the extract did not show any growth
inhibitory effect on lymphoblastic leukaemia cell (MOLT-4) Figure 3.10A).
The anti-proliferative activities of the crude whelk GAG extracts on the two
leukaemia cell lines compare favourably with the cisplatin positive control and the low IC50
observed for K562 suggests the crude whelk GAG extracts would show promise as the basis
for an anti-leukemia drug, based on the recommendation of the standard National Cancer
Institute criteria. More importantly, the different anticancer activities display by the crude
whelk GAG extracts on these two cell lines also suggests that the whelk derived GAG’s
could be selective for certain cell types and this selectivity may well be important in targeting
the effects of these molecules towards tumour cells.
134
A
0
0.2
0.4
0.6
0.8
1
1.2
1.4
0 0.39 0.78 1.56 3.12 6.25 12.5 25Absor
bance
after
96 ho
urs inc
ubati
on
Concentration in µM/ml
Antiproliferative effect of cisplatin on K562 Leukemia cell line
Cisplatinum
0
0.2
0.4
0.6
0.8
1
1.2
1.4
1.6
0 10 20 30 50 60 80 100
Absor
bance
after
96 ho
urs inc
ubati
on
Concentrations in µg/ml
Antiproliferative effect of whelk GAG on K562
leukemia cell line
Whelk GAG
B
0
0.2
0.4
0.6
0.8
1
1.2
1.4
1.6
0 10 20 30 50 60 80 100
Absor
bance
after
96 ho
urs
incub
ation
Concentrations in µg/ml
Proliferative effects of commercial GAGs on K562 leukemia cell line
HS
CS
Figure 3.10: MTT cell viability assay for MOLT-4 and K562 leukaemia cells after
treatment with whelk GAG extracts
Cells were incubated with various concentrations of GAGs for 96 hours after which time cell viability was
measured using an MTT assay (A) MOLT-4 leukaemia cells treated with crude whelk GAGs withcisplatin as a
positive inhibitory control, (B) K562 leukaemia cell line treated with crude whelk GAGs and cisplatin as a
positive control. Each value is presented as the mean SEM of three independent determinations. The bars in
each chart are presented as relative values in comparison to untreated cells.
Abbreviations- *-Significant (p≤0.05): **-Highly significant (p≤0.01)
** **
** ** ** ** ** ** ** **
** ** ** ** **
135
3.11 Effect of crude whelk GAG extracts on the growth of HeLa Cervical cells
The anticancer activity of whelk GAG mixture was also tested on the standard HeLa
cell line as this cell line is particularly susceptible to induction of apoptosis. The result shows
that crude whelk GAG mixture strongly inhibited the growth of the HeLa ovarian cell line
and its anticancer effects were more pronounced than on all other cancer cells investigated so
far in this study, with a typically recorded IC50 of 12μg/ml. Moreover, it is clear that the anti-
cancer activities of this whelk GAG mixure are greater than that observed for cisplatin anti-
cancer drug (Figure 3.11A-B).
Once again all commercial GAGs tested along with whelk crude GAGs did not
demonstrate any inhibitory effect on the HeLa cells proliferation: suggesting that the
inhibitory effect may be a unique feature of the GAG’s derived from whelks. This result also
suggests that this polysaccharide’s anti-cancer activity is stronger than cisplatinum anti-
cencer drug. In addition, the data suggests that the whelk derived GAG’s could be more
selective to this cell types than other cells tested and this selectivity may well be important in
targeting the effects of these molecules towards tumour cells.
136
0
0.2
0.4
0.6
0.8
1
1.2
1.4
1.6
0 0.39 0.78 1.56 3.12 6.25 12.5 25Abso
rban
ce a
fter
96
hour
s inc
ubat
ion
Concentrations in µM/ml
Anti proliferative effect of cisplatin on HeLa
cervical cell line
Cisplatinum
0
0.2
0.4
0.6
0.8
1
1.2
1.4
0 10 20 30 50 60 80 100
Abso
rban
ce a
fter
96
hour
s inc
ubat
ion
Concentrations in µg/ml
Anti proliferative effect of whelk GAG on HeLa
cervical cell
Whelk GAG
Figure 3.11: MTT cell viability assay for HeLa cervical cell after treatment with whelk
GAG extracts
Cells were incubated with various concentrations of GAGs for 96 hours after which time cell viability was
measured using an MTT assay with cisplatin as a positive inhibitory control. Each value is presented as the
mean SEM of three independent determinations. The bars in each chart are presented as relative values in
comparison to untreated cells.
Abbreviations: *- Significant (p≤): **-Highly significant (p≤0.01)
*
**
** **
*
137
3.12 Effect of crude whelk GAG mixtures on the growth of normal fibroblast cells
(3T3)
The effects of crude whelk GAGs on growth of normal fibroblast cells (3T3) was
measured using MTT colorimetric assay. Cells were exposed to different concentrations of
the crude whelk GAGs for 96 hours. Crude whelk GAG extracts did not show any growth
inhibitory effect on 3T3 cell proliferation (Figure 3.12). Moreover, the effects of crude whelk
GAGs on 3T3 cells compare favourably with the results obtained for commercial GAGs.
These results suggest that whelk derived GAG’s is selective against cancer cell types and at
least on a normal cell type and shows great potential in the treatment of this disease.
138
0
0.2
0.4
0.6
0.8
1
1.2
1.4
0 10 20 30 50 60 80 100Ab
sorb
ance
aft
er
96
ho
urs
incu
bat
ion
Concentrations in µg/ml
Anti proliferative effect of whelk crude GAGs on 3T3 fibroblast cell
wk
Figure 3.12: MTT cell viability assay of normal fibroblast 3T3 cells after treatment with
whelk GAGs extracts.
Cells were incubated with various concentrations of GAGs for 96 hours after which time cell viability was
measured using an MTT assay. Each value is presented as the mean SEM of three independent determinations.
The bars in each chart are presented as relative values in comparison to untreated cells.
139
3.13 Effect of Heparinase I, II, & III enzymes on anti-proliferative activity of whelk
GAG extracts using MDA468 and MDANQ01 breast cancer cell lines.
The crude whelk GAG extract was depolymerised with Heparinase I, II&III enzymes
to break the long linear chain polymer to smaller oligosaccharides chains, this has previously
been shown to destroy any GAG related biological activities. The oligosaccharide product
was then incubated with the two breast cancer cell lines (MDANQ01 and MDA 468) for 96
hours, as described under materials and methods. The results obtained showed a dramatic
reduction in the growth inhibitory effects of whelk GAG extracts on both breast cancer cell
lines (Figure 3.13A-B). These results suggest that the anticancer activities of these novel
GAG extracts appears to be connected to the intact linear polysaccharide chains that were
present in the crude GAG mixture.
140
A
0
0.2
0.4
0.6
0.8
1
1.2
1.4
0 1 3 5 10 20 50
Absor
bance
after
96 ho
urs in
cubati
on
Concentrations of both intact and enzymes treated GAGs in µg/ml
Anti proliferative effect of depolymerised whelk GAG on MDA468 breast cancer cell line
Crude whelk GAG
Whelk GAG treated with heparinase I -III
B
Anti proliferative effect of depolymerised whelk GAG on
MDANQ01 breast cancer cell line
0
0.2
0.4
0.6
0.8
1
1.2
1.4
1.6
0 1 3 5 10 20 50
Absor
banc
e afte
r 96 h
ours
incub
ation
Concentrations of both intact and enzymes
treated GAGs in µg/ml
Crude Whelk GAG
whelk GAG treated with heparinase I-
III
Figure 3.13: MTT cell viability assay for MDANQ01 and MDA468 breast cancer cells
after treatment with heparinase depolymerised whelk GAG extracts.
Cells were incubated with various concentrations of GAGs for 96 hours after which time cell viability was
measured using an MTT assay (A) MDA468 cells after treatment with whelk GAG Heparinase I-III enzyme
digest with cisplatin as a positive inhibitory control, (B) MDANQ01 cells treated with whelk GAG Heparinase
I-III enzyme digest with cisplatin as a positive inhibitory control. Each value is presented as the mean SEM of
three independent determinations. The bars in each chart are presented as relative values in comparison to
untreated cells.
Abbreviations: *-Significant (p≤0.05): **-Highly significant (p≤0.01)
*
** ** **
*
** **
141
3.14 Cell cycle analysis of MDANQ01 cells after treatment with crude whelk GAG
extracts
Flow cytometry was used to investigate the effects of the whelk GAG extracts on the
progression of the cell cycle. Cells exposed to either 20ug/ml or 50ug/ml whelks GAG’s
showed perturbation of MDANQ01 cell’s cycle after 24-72 hours exposure to the crude
extract.
Whelk GAGs induced cell cycle arrest of MDANQ01 cells at both S and G2M phases
was observed as shown in Figure 3.14A-C. This brought about a significant accumulation of
cells at S and G2/M phases leading to the subsequent reduction of number of cells in G1
phase. 24 hours treatment of MDANQ01 cells with 50µg/ml whelk GAGs caused a marginal
increased in the number of cells at G2/M-phase from 26.97% ± 6.28 (control) to 29.16% ±
0.1) (50 µg/ml wk). At 48 h the cell population at S-phase (Figure 3.14A-C) increased from
20.48% ±8.19 (control) to 26.76% ±2.26 (50 µg/ml whelk). Similarly lower concentrations of
whelk GAGs disrupted MDANQ01 cell cycle progression at both S and G2/M.The longest
incubation time (72 hours) with low doses of the crude GAGs (Figure 3.14A-C) significantly
altered the cell cycle by inducing a more than two fold increase in the percentage of cell
population at the G2/M-phase (p<0.02). [Control cell (18.82% ± 1.70)] treated cell (37.39% ±
3.48].
142
A
24 hours Untreated Treated
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*
Cell cycle arrest caused by whelk GAG treatment on MDANQ01 breast cancer cell line
143
Figure 3.14: Cell cycle analysis of MDANQ01 breast cancer cell line following treatment
with crude whelk GAG extract.
MDANQ01 breast cancer cells were treated with PI stain and subjected to cell cycle analysis by flow cytometry
(A). Charts showed averages of three independent experiments after treatment with or without crude whelk
GAGs. (B) Flow cytometry of MDANQ01 cells after 24 hours incubations with or without crude whelk GAGs.
(C) Flow cytometry of MDANQ01 breast cancer cells after 48 hours incubation with or without crude whelk
GAGs and (D) Flow cytometry of MDANQ01 breast cancer cells after 72 hours incubation with or without
crude whelk GAGs.
Abbreviations: *- Significant (p≤0.05)
144
3.15 Cell cycle analysis of MDA468 breast cancer cell lines after treatment with
crude whelk GAG extracts
Whelk GAGs treatment also caused significant cell cycle disruptions in the MDA468
breast cancer cell line in a similar manner to that observed in the MDANQ01 cells. Cell cycle
disruptions were observed at both S and G2/M phases (see Figure 3.15A-C). Higher
concentrations of whelk GAGs (50µg/ml) also induced a time-dependent DNA disruptive
effect on MDA468 cells as shown in Figure 3.15A-B. A short hour (48 hours) incubation of
the crude whelk GAG extracts with MDA468 cells induced cell accumulation at G2/M;
however, these differences were not statistically significant (p>0.05) when compared with the
corresponding values of the control.
The longer 72 hours incubations of the cells with high doses of crude GAGs
significantly altered the cell cycle by inducing more than a two-fold increase in the
percentage of cell population at the S-phase (p<0.02). Crude whelk GAG extracts increased
cell population at G2/M-phase from 24 ± 4.8 % (control) to 31 ± 3.4% (50µg/ml whelk) after
48 hours incubation but this increase is not statistically significant (p<0.14).
145
A
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File: Dorcas MDAnq01 10 WK +FCS 2. 24.21.02.12_027 Date: 21-02-2012 Time: 16:30:28 Particles: 569561 Acq.-Time: 53 s Concentration: 500 / ml
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G1
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*
Cell cycle arrest induced by whelk GAG treatment on MDA468 breast cancer
cell line
146
Figure 3.15: Cell cycle analysis of MDA468 breast cancer cell line following treatment
with crude whelk GAG extract.
MDA468 breast cancer cells were stained with PI stain and subjected to cell cycle analysis by flow cytometry
(A). Charts showed averages of three independent experiments after treatment with or without crude whelk
GAGs (B) Flow cytometry of MDA468 breast cancer cells after 48 hours incubation with or without crude
whelk GAGs and (C) Flow cytometry of MDA468 breast cancer cells after 72 hours incubation with or without
crude whelk GAGs.
Abbreviations: *- Significant (p≤0.05)
.
.
147
3.16 Effects of crude whelk GAG mixtures on the induction of apoptosis in MDA468
breast cancer cells
Previous investigations revealed that whelk GAGs induced cell death in MDA468
breast cancer cells; however, the mechanism of cell death induced by this crude
polysaccharide was not yet known. An Annexin V-FITC Apoptosis Detection Kit was used in
order to elucidate the mechanism of cell death induced by whelk GAG extracts. The two cell
lines were incubated with varying concentrations of the whelk GAGs at different time
intervals and the apoptosis determination was carried out as described under the materials and
methods section. The results reveal that high concentration (50µg/ml) of the whelk GAG
extract appears to have caused the breast cancer cells death by inducing apoptosis (late
apoptosis) in proportion to the rate of cell death caused by the crude extract on the cells
Figure 3.16A-C).
Whelk GAG extracts (50 µg/ml) increased the percentage of cells stained positive for
both Annexin V-FITC and PI after 24 hours treatment from 16.48 (control) to 28.40
(50µg/ml). 48-hour incubations with the whelk GAGs also slightly increased the number of
cells stained with annexin V-FITC from 1.64 % (control) to 2.4 % (50µg/ml). However there
were signs of substantial cell lysis at this time point. Moreover, the number of cells stained
positive for both Annexin V-FITC and PI increased marginally from 8.2 % (control) to 12.89
% (50µg/ml). However, lower concentration (20µg/ml) of the whelk GAG extract did not
show any apoptotic effect on MDA468 cell line: both 8 and 72 hours incubations of the cells
with the crude extract did not show any noticeable apoptotic effect on the two cell lines
(results not shown).
In addition to the late apoptotic effect of the extract on MDA468 breast cancer cell,
there was a false apoptotic effect observed in the control cells 24 hours after incubation,
148
likely caused by trypsinisation of the cells after incubation. In order to eliminate this false
apoptotic effect, both the treated and untreated cells were stained with DAPI and viewed
under the fluorescent microscope as described under the materials and methods.
149
obtained are discussed in the following section.
B 24 hours Untreated Treated
24 hours Untreated Treated
C 48 hours Untreated Treated
A
*
24 hours 48 hours
Apoptosis induced by whelk GAG treatment on MDA468 breast cancer cell line
150
Figure 3.16: Detection of Apoptotic MDA468 breast cancer cells treated with crude
whelk GAG extracts by Annexin V Staining.
MDA468 breast cancer cells were treated with crude whelk GAGs for 24 and 48 hours and then stained using
Annexin V-FITC and PI provided in the Annexin V-FITC Apoptosis Detection Kit (see materials and methods).
The combination of Annexin V-FITC and PI allows for the distinction between early apoptotic cells (annexin V-
FITC positive), late apoptotic and/or necrotic cells (Annexin V-FITC and PI positive), necrotic (PI stained
positive) and viable cells (unstained). (A) MDA468 cell treated with or without crude whelk GAGs for 24 and
48 hours respectively. (B) MDA468 cell treated with or without crude whelk GAGs for 24 hours. (C) MDA468
cell treated with or without crude whelk GAGs for 48 hours.
Abbreviations: *- Significant (p≤0.05)
151
3.17 Flow cytometry and Annexin V-FITC apoptosis detection of MDANQ01 cells
following incubation with whelk GAG extracts
Whelk GAGs induced cell death in MDANQ01 breast cancer cells; however, the
mechanism of cell death induced by this crude GAG required further study. In order to
elucidate the mechanism of cell death induced by crude whelk GAGs, Annexin V-FITC
Apoptosis Detection Kit was utilised (see materials and methods). High concentration
(50µg/ml) of crude whelk GAGs induced time-dependent apoptosis on MDANQ01 cells
(Figure 3.17A-C). 24-hour incubation of the crude whelk GAG extracts with the cells,
increased the number of cells stained with annexin V-FITC from 1.02 % (control) to 2.84 %
(50 µg/ml) and the number of cells stained with both Annexin V-FITC and PI was also
increased from 7.07 % (control) to 15.16 % (50 µg/ml).
Similarly, 48-hour incubation of the whelk GAG extract also induces apoptosis on
MDANQ01 cells but the apoptotic effect was slightly reduced than the observations made at
24 hours. At 48 hours, the number of cells stained with annexin V-FITC increased from
2.99% (control) to 5.92 (50µg/ml) and those cells stained with both Annexin V-FITC and PI
also increased from 9.28 % (control) to 13.66 % (50µg/ml). However, lower concentration
(20µg/ml) of the crude extract did not show any apoptotic effect on this cell line. Both 8 and
72 hours incubations of the cells with the crude extract did not show any noticeable apoptotic
effect on MDANQ01 cell line (results not shown).
Similarly, a false apoptotic effect was observed in the control cells, which may be
caused by the trypsinisation’s step draw back of the cells after incubation. In order to rule out
this false apoptotic effect, both the treated and untreated cells were also stained with DAPI
and viewed under the fluorescent microscope, as described under the materials and methods.
The results obtained are discussed later in this section.
152
A
B 24 hours Untreated Treated
C 48 hours Untreated Treated
Apoptosis induced by whelk GAG treatment on MDANQ01 breast cancer
cell line
24 hours 48 hours
*
153
Figure 3.17: Detection of Apoptotic MDANQ01 breast cancer cells treated with crude
whelk GAG extracts by Annexin V Staining.
MDANQ01 breast cancer cells were treated with crude whelk GAGs for 24 and 48 hours and then stained using
Annexin V-FITC and PI provided in the Annexin V-FITC Apoptosis Detection Kit (see materials and methods).
The combination of Annexin V-FITC and PI allows for the distinction between early apoptotic cells (annexin V-
FITC positive), late apoptotic and/or necrotic cells (Annexin V-FITC and PI positive), necrotic (PI stained
positive) and viable cells (unstained). (A) MDANQ01 cell treated with or without crude whelk GAGs for 24 and
48 hours respectively. (B) MDANQ01 cell treated with or without crude whelk GAGs for 24 hours. (C)
MDANQ01 cell treated with or without crude whelk GAGs for 48 hours.
Abbreviations: *- Significant (p≤0.05)
154
3.18 Assessment of apoptosis using DAPI flourescent microscopy following treatment
of MDA468 breast cancer cell with Crude whelk GAG extracts
To confirm whether the anti-proliferative effect of whelk GAG extracts on MDA468
breast cancer cell line was due to apoptosis; cells were incubated with or without crude whelk
GAGs, stained with DAPI stain and the cells morphology examined under a fluorescent
microscope. MDA468 cells were treated with 50 μg/ml of crude whelk GAGs or negative
control (FCS media) for 24 and 48 hours and subsequently analysed by DAPI staining.
Control cells incubated with media and without crude whelk GAGs showed no signs of
apoptosis or oncosis and exhibited brightly fluorescing round, blue-stained nuclei (Figure
3.18A-B). In contrast, those cells treated with crude whelk GAGs for 24 and 48 hours showed
a number of cells with condensed and fragmented nuclei, an indication of apoptosis (Figure
3.18A-B).
Trypsinisation, which is known to cause membrane damage, is one of the major steps
involved in annexin V-FITC apoptosis detection assay. It may be responsible for some false
anexin V-FITC positive staining observed in the untreated group. The above result obtained
from DAPI stain confirms this hypothesis and shows clearly that the control group showed no
induction of any apoptosis. This result also confirms that crude whelk GAG extracts induces
apoptosis on MDA468 breast cancer cell. Therefore, the combined results of apoptosis
detections by annexin V-FITC and DAPI stains suggest that the breast cancer cell death
caused by crude whelk GAGs treatment was caused in part by apoptosis.
155
A 24 hours Untreated Treated
B 48 hours Untreated Treated
156
Figure 3.18: Detection of apoptotic MDA468 cells by DAPI fluorescent microscopy
following treatment with crude whelk GAG extracts.
MDA468 cells treated with crude whelk GAGs were stained and morphology of apoptotic cell nuclei was
observed by DAPI staining using a fluorescence microscope. Nuclei were stained with DAPI (blue). Images
were photographed at the same exposure time under a x40 objective with Hamatsu 1394 ORCA-285 camera.
(A) MDA468 cells treated with or without crude whelk for 24 hours. (B) MDA468 cells treated with or without
crude whelk GAGs for 48 hours. Arrows represent the condensed or fragmented nuclei of cells.
3.19 Assessment of apoptosis using DAPI flourescent microscopy following treatment
of MDANQ01 breast cancer cell with Crude whelk GAG
Similarly, to confirm whether the reduced cell growth observed in MDANQ01 cell
line treated with crude whelk GAGs was due to apoptosis as revealed by annexin V-FITC
apoptosis detection. MDANQ01 cells treated with or without 50μg/ml of crude whelk GAGs
for 24 and 48 hours were stained with DAPI and cell morphology examined under fluorescent
microscope. Control cells incubated with media without crude whelk GAGs showed no signs
of apoptosis or oncosis and exhibited brightly fluorescing round, blue-stained nuclei (Figure
3.19A-B). However, the treated cells showed a numbers of cells with condensed and
fragmented nuclei, an indicator of apoptosis (Figure 3.19A-B).
Furthermore, this result confirms that crude whelk GAG extracts induce apoptosis on
MDANQ01 cells. Therefore, the combined results of apoptosis detections by annexin V-
FITC and DAPI staining suggest that the anti-proliferative activity of the crude whelk GAGs
on MDANQ01 breast cancer cells was partly due to apoptosis.
157
nnnm
Figure 3.19: Detection of apoptotic MDANQ01 cells treated with crude whelk GAG
mixtures by DAPI fluorescent microscopy.
A 24 hours Untreated Treated
B 48 hours Untreated
Treated (48 hours)
48 hours Untreated Treated
B
158
Figure 3.19: Detection of apoptotic MDANQ01 cell treated with crude whelk GAG
mixtures by DAPI fluorescent microscopy
MDANQ01 cells treated with crude whelk GAGs were stained with DAPI and morphology of apoptotic cell
nuclei was observed by DAPI staining using a fluorescence microscope. Nuclei were stained with DAPI (blue).
Images were photographed at the same exposure time under a x40 objective with Hamatsu 1394 ORCA-285
camera. (A) MDANQ01 cells treated with or without crude whelk for 24 hours. (B) MDANQ01 cells treated
with or without crude whelk GAGs for 48 hours. Arrows represent the condensed or fragmented nuclei of cells
159
3.20 Assessment of apoptosis using annexin V-FITC apoptosis detection following
treatment of HeLa cells with crude whelk GAG extracts
Preliminary studies reveal that crude whelk GAGs cause cell death in HeLa cells but
the mechanism of this cell death is not yet known. This study was performed to elucidate the
mechanism of cell death induced by crude whelk GAGs on HeLa ovarian cells using an
Annexin V-FITC Apoptosis Detection Kit. HeLa cells are one of the most susceptible cells to
apoptosis, as demonstrated and confirmed in this sudy. The apoptotic effects of whelk GAGs
were more pronounced and better established with this cell line than that seen in either the
leukaemia or breast cancer cell lines. 24-hour incubation of the crude whelk extracts with
HeLa cells induce almost 50% apoptosis (late apoptosis) with an additional 10% early
apoptosis detected and this differences were highly significant (p=0.000) when compared
with the corresponding values of the control. Moreover, a number of cell deaths were caused
by necrosis, as illustrated in (Figure 3.20A-C). Additionally, 48-hour incubation of the crude
whelk GAGs with HeLa cells also induced almost 70% late apoptosis and almost 10% early
apoptosis, with a few cells (< 10%) affected by necrosis (Figure 3.20A-C). Small amounts of
positive apoptosis and necrosis were observed in the untreated control cells. This was easily
resolved by fluorescent microscopy and DAPI staining, which reveals no false positive for
either necrosis or apoptosis detection in the untreated cells.
160
Fig.24 hours
A
B 24 hours Untreated Treated
C 48 hours Untreated Treated
48 hours
Apoptosis induced by whelk GAG treatment on HeLa cervical cell line
24 hours
**
*
**
*
161
Figure 3.20: Detection of Apoptosis in HeLa cells by Annexin V Staining following
treatment with whelk GAG extracts.
HeLa cells were treated with crude whelk GAGs for 24 and 48 hours and then stained using Annexin V-FITC
and PI provided in the Annexin V-FITC Apoptosis Detection Kit. The combination of Annexin V-FITC and PI
allows for the distinction between early apoptotic cells (annexin V-FITC positive), late apoptotic and/or necrotic
cells (Annexin V-FITC and PI positive), necrotic (PI stained positive) and viable cells (unstained). (A) HeLa
cell treated with or without crude whelk GAGs for 24 and 48 hours respectively. (B) HeLa cell treated with or
without crude whelk GAGs for 24 hours. (C) HeLa cells treated with or without crude whelk GAGs for 48 hours
Abbreviations: *-Significant (p≤0.05)
3.21 Assessment of apoptosis using DAPI flourescent microscopy following treatment
of HeLa cells with whelk GAGs
Apoptotic effects of crude whelk GAGs on HeLa cervical cells were confirmed as
follows: Cells treated with 50μg/ml of crude whelk GAGs or negative control (FCS media)
for 24 and 48 hours were stained with DAPI and viewed under fluorescent micrope. Control
cells incubated in ordinary FCS media without crude whelk GAGs exhibited no signs of
apoptosis and exhibited brightly fluorescing round, blue-stained nuclei (Figure 3.21A-B). In
contrast, cells treated with whelk GAG extracts showed a number of cells with condensed
and fragmented nuclei; a clear indication of apoptosis induction (Figure 3.21A-B). This
result confirms that whelk GAG extracts induce apoptosis with the HeLa cells. Both the
DAPI and annexin V-FITC results suggest that cell growth inhibitory activity of whelk GAGs
on HeLa cells was due in part to apoptosis.
162
A 24 hours Untreated Treated
B 48 hours Untreated
B 48 hours Untreated Treated
B
163
Figure 3.21: Detection of apoptotic HeLa cells by DAPI fluorescent microscopy
following treatment with whelk GAG
HeLa cells, treated with crude whelk GAGs, were stained with DAPI and the morphology of apoptotic cell
nuclei was observed by DAPI staining using a fluorescence microscope. Nuclei were stained with DAPI (blue).
Images were photographed at the same exposure time under a x40 objective with Hamatsu 1394 ORCA-285
camera. (A) HeLa cells treated with or without crude whelk for 24 hours. (B) HeLa cells treated with or without
crude whelk GAGs for 48 hours. Arrows represent the condensed or fragmented nuclei of cells.
164
3.22 Fractionation of whelk GAG extracts by ion-exchange chromatography
Crude whelk GAG extracts were next subjected to ion-exchange chromatography in
order to identify the biologically active component. Ion-exchange chromatography is used
routinely to separate GAG mixtures into their respective GAG family members; for example,
HS, CS and DS. Six major peaks were identified, when the whelk GAG extracts were
subjected to ion-exchange separation; each peak was believed to contain different GAGs
family members (Figure 3.22). Peaks were designated, A-F, in order of increased elution time
(table 1). In some preparations fraction D was absent; however, the remainders of the
fractions were consistently present. When assayed in the MTT assay against both breast
cancer cell lines, only a single fraction (E) had any significant anti-proliferative effect (Figure
3.23)
165
Figure 3.22: Ion-exchange chromatography elution profile for whelk GAG extracts.
Samples were applied to a DEAE-Sephadex ion-exchange column and resolved using a linear 0-3 M NaCl
gradient in 50mM sodium phosphate buffer pH 7.0 at a flow rate of 1ml/min for 100 min. Fractions were
collected and the absorbance monitored at a wavelength of 254nm. Fractions were pooled as indicated, desalted
and lyophilised before further analysis.
Fractionation of whelk GAG by anion exchange chromatography
166
Table 2: Ion-exchange chromatographic separation of whelk GAG extracts
Fraction
name
Fraction
number
GAGs type Percentage
yield (%)
Elution time
(minutes)
Nacl
gradient (M)
A 27-37 HS-like 19.90 27-37 0.9-1.24
B 39-47 CS/DS-like 13.50 39-47 1.26-1.62
C 49-62 CS/DS-like 18.00 49-62 1.63-2.1
D 65-73 Unknown 16.00 65-73 2.14-2.5
E 75-88 HS-like 23.30 75-88 2.56-2.9
F 89-94 Unknown 9.30 89-94 2.91-3.0
Samples were applied to a DEAE-Sephadex ion-exchange column and resolved by a linear 0-3 M NaCl gradient
in 50mM sodium phosphate buffer pH 7.0 at a flow rate of 1ml/min for 100 min. Fractions were collected and
the absorbance monitored at wavelengths of 254nm. Fractions were pooled as indicated, desalted and
lyophilized before further analysis.
167
Table 3: Summary of biological effects of whelk GAGs
MDA468
breast
cancer cell
line
MDANQ0
1 breast
cancer cell
line
K562
erythrocyti
c leukemia
cell line
MOLT-4
leukemia
cell line
HeLa
cervical
cell line
3T3
normal
fibrobla
st cell
line
Proliferati
ve assay
Inhibited
cell growth
Inhibited
cell growth
Inhibited
cell growth
Inhibited
cell
growth
Inhibited
cell
growth
Suppor
ted cell
growth
IC50 70.94µg/ml 25.14µg/ml 14µg/ml 41.11µg/
ml
12µg/ml -
Cell cycle
arrest
Induced
cell cycle
arrest at
both S and
G2/M
phase
Induced
cell cycle
arrest at
both S and
G2/M
phase
- - - -
Apoptosis
detection
assay
Induced
late
apoptosis
Induced
late
apoptosis
- - Induced
late
apoptosis
-
Note: Also included in this section was proliferative effect of depolymerised whelk GAG on
both MDA468 and MDANQ01 breast cancer cell lines.
168
Section 3C
Biological activities of purified whelk
fraction E
169
3.23 Effect of purified whelk fraction E on the growth of MDANQ01 breast cancer
cells
Fraction E samples showed significant (p<0.05) growth inhibitory effects on
MDANQ01 breast cancer cells proliferation (Figure 3.23A) after 96 hours incubation as
described under materials and methods section. The growth inhibitory effects of fraction E on
MDANQ01 was similar to that observed for crude whelk GAGs extracts but the recorded
IC50 (41.89 μg/ml) was higher than what was recorded for crude whelk GAGs (25.14 μg/ml).
However, the growth inhibitory effect of fraction E was more pronounced with higher
concentrations (50-100 μg/ml) than the lower concentrations (10-30 μg/ml).
In addition to the above result, other purified whelk fractions (A,B,C,& F) and
commercial GAGs were also tested along with fraction E. Interestingly none of them showed
any growth inhibitory effect on MDANQ01 breast cancer cells proliferation (Figure 3.23B)
170
0
0.2
0.4
0.6
0.8
1
1.2
0 10 20 30 50 60 80 100Absor
bance
after
96 ho
urs
incub
ation
Concentrations in µg/ml
Proliferative effects of purified whelk fractions and commercial GAGs on MDANQ01 breast cancer cell line
Fraction A
Fraction B
Fraction C
Fraction F
CS
HS
B
0
0.2
0.4
0.6
0.8
1
1.2
1.4
1.6
0 10 20 30 50 60 80 100
Abso
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e afte
r 96 h
ours
incub
ation
Concentrations in µg/ml
Antiproliferative effect of purified whelk GAG on MDANQ01 breast cancer cell line
Whelk GAGs
Fraction E
Figure 3.23: MTT cell viability assay for MDANQ01 breast cancer cells after treatment
with GAG mixtures and purified whelk fraction E.
Cells were incubated with various concentrations of GAGs for 96 hours after which time cell viability was
measured using an MTT assay (A) MDANQ01 breast cancer cell line treated with crude whelk’s purified
fractions and commercial GAGs (B) MDANQ01 breast cancer cells treated with fraction E and crude whelk
GAGs. Each value is presented as the mean SEM of three independent determinations. The bars in each chart
are presented as relative values in comparison to untreated cells.
Abbreviations: *-Significant (p≤0.05): **-Highly significant
* ** ** ** **
171
3.24 Effect of purified whelk fraction E on MDA468 breast cancer cell proliferation
Fractions E also showed dose-dependent growth inhibitory effects on MDA468 breast
cancer cell line (Figure 3.24A) after 96 hours treatment (see materials and methods section).
Its growth inhibitory effect on MDA468 compares favourably to the effect of the crude whelk
GAG extracts with a lower recorded IC50 of 45.98μg/ml against an IC50 of 70.96 μg/ml
recorded for crude whelk GAGs. Similarly, higher concentrations (50-100 μg/ml) of fraction
E show more effective growth inhibitory activity against MDA468 than their lower
concentrations (10-30 μg/ml) counterpart (Figure 3.24A).
However, other purified whelk fractions (A, B, C & F) and commercial GAGs did not reveal
any growth inhibitory activity against MDA468 cells (Figure 3.24B)
172
A
0
0.2
0.4
0.6
0.8
1
1.2
0 10 20 30 50 60 80 100
Absor
bance
after
96 ho
urs
incub
ation
Concentrations in µg/ml
Proliferative effects of purified whelk fractions and commercial GAGs on MDA 468 breast cancer
cell lineFraction A
Fraction B
Fraction C
Fraction F
CS
HS
B
0
0.2
0.4
0.6
0.8
1
1.2
1.4
1.6
0 10 20 30 50 60 80 100Absor
bance
after
96 ho
urs
incub
ation
Concentrations in µg/ml
Anti proliferative effects of fraction E and whelk GAGs on MDA468 breast cancer cell line
Whelk GAGs
Fraction E
Figure 3.24: Concentration-dependent effect of purified whelk GAG fraction E on
MDA468 breast cancer cell viability.
Cells were incubated with various concentrations of cockle GAGs for 96 hours after which time cell viability
was measured using an MTT assay (A) Cells treated with commercial GAGs and whelk’s purified fractions (B)
Cells treated with fraction E and crude whelk GAG extracts. Each value is presented as the mean SEM of three
independent determinations. The bars in each chart are presented as relative values in comparison to untreated
cells.
Abbreviations: **- Highly significant (p≤0.01)
* *
** **
**
173
3.25 Cell cycle analysis of the MDANQ01 breast cancer cell line after treatment with
purified whelk fraction E
Whelk fraction E induced cell cycle arrest on MDANQ01 cells at both S and G2/M
phases as shown in Figure 3.25A-C. It caused significant accumulations of cells at S and
G2/M phases, leading to the subsequent reduction in the overall number of cells in G1 phase.
After 48 hours treatment with 50µg/ml whelk fraction E, the percentage of cell population at
S-phase increased from 20.48 % (control) to 25.06 % (50 µg/ml fraction E). At 72 hours, the
cell population at G2/M-phase increased from 21.27 % (control) to 38.46 % (Figure 3.25A-C)
This result suggests that purified fraction E partly elicits its anti-proliferative activity
on MDANQ01 breast cancer cells by inducing cell cycle arrest at S and G2/M-phase.
174
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48 hours Untreated Treated
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*
Cell cycle arrest caused by fraction E treatment on MDANQ01 breast cancer cell line
175
Figure 3.25: Cell cycle analysis of MDANQ01 breast cancer cell line following treatment
with purified whelk fraction E.
MDANQ01 breast cancer cells were stained with PI stain and subjected to cell cycle analysis by flow cytometry
(A). Charts showed averages of three independent experiments after treatment with or without purified whelk
fraction E (B) Flow cytometry of MDANQ01 breast cancer cells after 48 hours incubation with or without
purified whelk fraction E and (C) Flow cytometry of MDANQ01 breast cancer cells after 72 hours incubation
with or without purified whelk fraction E.
Abbreviations: *- Significant (p≤0.05)
3.26 Cell cycle analysis of the MDA468 cell line after treatment with Purified whelk
fraction E
Cells exposed to 50ug/ml whelks fraction E showed perturbation of MDA468 cell’s
cycle after 24-72 hours exposure to the purified extract.
Whelk fraction E induced mild cell cycle arrest of MDA468 cells at both S and G2/M phases
as shown in Figure 3.26A-C. After 24 hours treatment with 50µg/ml whelk fraction E,
MDA468 cells population at S-phase increased from 21.94% (control) to 29.19% (50 µg/ml
fraction E). 72 hours incubation of the cell with purified fraction E also increased the cell
population at G2/M from 25.75% (control) to 35.75% (50 µg/ml fraction E). However, 48-
hour incubation of the purified fraction E with MDA468 cell did not have any effect on the
cell cycle.
The purified fraction E showed consistent DNA disruptive effect on both breast cancer
cell lines and these results suggest that the purified fraction E induces growth inhibitory
effect on the MDA468 and MDANQ01 breast cancer cells via cells cycle arrest at S and
G2/M-phase.
176
A
24 hours Untreated Treated
B
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Cell cycle arrest caused by fraction E treatment on MDA468 breast cancer cell line
*
177
Figure 3.26: Cell cycle analysis of MDA468 breast cancer cell line following treatment
with purified whelk fraction E.
MDA468 breast cancer cells were stained with PI stain and subjected to cell cycle analysis by flow cytometry
(A). Charts showed averages of three independent experiments after treatment with or without purified whelk
fraction E (B) Flow cytometry of MDANQ01 breast cancer cells after 24 hours incubation with or without
purified whelk fraction E and (C) Flow cytometry of MDANQ01 breast cancer cells after 72 hours incubation
with or without purified whelk fraction E.
Abbreviations: *- Significant (p≤0.05)
72 hours Untreated Treated
B
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3.27 Purified whelk fraction E induces mild apoptosis and necrosis on MDANQ01
breast cancer cells (revised Annexin V-FITC apoptosis detection assay results).
High concentration (100µg/ml) of purified whelk fraction E induces mild apoptosis
and necrosis on MDANQ01 cell (Figure 3.28 (A-B). 24-hour incubation of the purified
fraction with the cells increased the number of cells stained with Annexin V-FITC from 1.02
% (control) to 2.01 % (100µg/ml). The number of cells stained with both Annexin V-FITC
and PI also increased from 7.07 % (control) to 9.3 % (100µg/ml). In addition, this extract
induces mild necrosis on MDANQ01 cells: the cell stained with PI increased from 6.47 %
(control) to 7.56 % (100µg/ml).
However, lower concentration (20-50µg/ml) of the purified fraction did not yield any
apoptotic effect on this cell line: both 8 and 72-hour incubations of the cells with the purified
fraction did not exhibit any noticeable apoptotic effect on MDANQ01 cell line (results not
shown).
179
A
Figure 3.27: Detection of Apoptotic MDANQ01 breast cancer cells treated with purified
whelk fraction E by Annexin V Staining.
MDANQ01 cells were treated with purified whelk fraction E for 24 hours and then stained using Annexin V-
FITC and PI provided in the Annexin V-FITC Apoptosis Detection Kit (see materials and methods). The
combination of Annexin V-FITC and PI allows for the distinction between early apoptotic cells (annexin V-
FITC positive), late apoptotic and/or necrotic cells (Annexin V-FITC and PI positive), necrotic (PI stained
6t66positive) and viable cells (unstained). (A) MDANQ01 cell treated with or without purified whelk fraction E
24 hours. (B) Flow cytometry of MDANQ01 treated with or without purified whelk fraction E for 24 hours.
24 hours Untreated Treated
B
Apoptosis induced by fraction E treatment on MDANQ01breast cancer
cell line
180
3.28 Annexin V-FITC apoptosis assay of the MDA468 breast cancer cell line following
treatment with purified whelk fraction E
Purified fraction E induces time-dependent apoptosis on MDA468 cells (Figure
3.28A-C). 24 hours incubations of purified fraction E with the cells increased the number of
cells stained with both Annexin V-FITC and PI from 16.48 % (control) to 20.96 %
(50µg/ml). Similarly, 48-hour incubations of the purified fraction E also induce late apoptosis
on MDANQ01 cells but the apoptotic effect was more pronounced than that observed at 24
hours. At 48 hours, the number of cells stained with Annexin V-FITC and PI increased from
8.2 % (control) to 14.16 % (50µg/ml). In addition to the apoptotic effect of the purified
fraction on MDA468 cells, there was also an increase in the number of cells stained with PI;
an indication of necrosis. At 48 hours, the number of cells stained with PI increased from 4.0
% (control) to 7.4 % (50µg/ml).
However, other concentrations (20 and 100µg/ml) of the purified fraction did not
show any apoptotic effect on this cell line: both 8 and 72-hour incubations of the cells with
the crude extract did not show any noticeable apoptotic effect on the MDA468 cell line
(results not shown) presumable due to the extent of cell death seen in the higher doses.
The observed apoptotic and necrotic effect of the purified fraction E on both breast cancer
cells suggest the possible growth inhibition of these cells proliferation was caused by
apoptosis and oncosis.
181
24 hours 48 hours
A
24 hours Untreated Treated
B
48 hours Untreated Treated
C
Apoptosis induced by fraction E treatment on MDA468 breast cancer cell line
182
Figure 3.28: Detection of time-dependent Apoptotic MDA468 breast cancer cells treated
with purified whelk fraction E by Annexin V Staining.
MDA468 cells were treated with purified whelk fraction E for 24 and 48 hours and then stained using Annexin
V-FITC and PI provided in the Annexin V-FITC Apoptosis Detection Kit (see materials and methods). The
combination of Annexin V-FITC and PI allows for the distinction between early apoptotic cells (annexin V-
FITC positive), late apoptotic and/or necrotic cells (Annexin V-FITC and PI positive), necrotic (PI stained
positive) and viable cells (unstained). (A) MDA468 cells treated with or without purified whelk fraction E for
24 and 48 hours. (B) Flow cytometry of MDA468 treated with or without purified whelk fraction E for 24 hours
and (C) Flow cytometry of MDA468 treated with or without purified whelk fraction E for 48 hours.
183
Table 4: Summary of biological effects of fraction E
MDA468 breast
cancer cell line
MDANQ01 breast
cancer cell line
3T3 normal
fibroblast cell line
Proliferatve assay Inhibited cell growth Inhibited cell growth Supported cell
growth
IC50 45.98µg/ml 41.89µg/ml -
Cell cycle arrest Induced cell cycle
arrest at both S and
G2/M phase
Induced cell cycle
arrest at both S and
G2/M phase
-
Apoptosis detection
assay
Induced late
apoptosis
Induced late
apoptosis
-
184
Section 3D
Characterisation and purification results
for cockle GAGs
185
3.29 Assignment of unsaturated CS dissacharides from cockle GAG extracts.
In order to ascertain the presence of CS/DS-like disaccharides in crude cockle
GAG extracts, samples were degraded by chondroitinase-ABC lyase, and the unsaturated
disaccharides produced were resolved by SAX-HPLC. The major disaccharides produced
were non and mono-sulfated Δ UA 1 → 3GalNAc, Δ UA 1 → 3GalNAc6S and Δ UA 1 →
3GalNAc4S (Table 5). Commercial CS was analysed along side with samples for qualitative,
and standardisation purposes and the digestion was monitored at 232 nm to assess when
completion had occurred (Figure 3.29)
The elution profiles for crude cockle GAG extracts were compared with the reference
chromatogram and they showed that the crude cockle GAG extracts contains both CS\ DS
(Figure not shown.).
The first peak (I) with retention time 16 minutes is assigned to non-sulfated
disaccharide (ΔDi-0S) composed ΔUA→3GalNAc. The second peak (II) with retention time
19 minutes is assigned to mono-sulfated disaccharide (ΔDi-6S) composed of
ΔUA→3GalNAc (6S). The third peak (III) with retention time 20 minutes is assigned to
mono-sulfated disaccharide (ΔDi-4S) composed of ΔUA→3GalNAc (4S). The percentage
compositions of each disaccharide peak from ABC lyase digested cockle GAG samples using
the peak area were 60%, 20% and 20% respectively. Other unidentified peaks were also
eluted along with the disaccharides which may suggest partial digestion or resistance to the
enzyme’s action. This result suggests that crude cockle GAG mixture contain CS/DS GAGs.
186
Table 5: Disaccharides compositions of CS/DS-like glycans found in cockle GAG
mixtures
Disaccharides Cockle GAG mixtures
disaccharide
compositions in %
Commercial CS
GAG disaccharide
compositions in %
Retention
time
(Rt) in
minutes
Δ UA-GalNac 60 Not detected 16
Δ UA-GalNac (6S) 20 27 19
Δ UA-GalNac (4S) 20 73 20
Δ UA (2S)-GalNac Not detected Not detected
Δ UA-GalNac (4S,6S) Not detected Not detected
Δ UA (2S)-GalNac (6S) Not detected Not detected
Δ UA2S-GalNac4S Not detected Not detected
The percentage compositions of each disaccharides peak was calculated by using peak area
values obtained from SAX-HPLC software.
187
Figure 3.29: Kinectic of chondroitinase ABC enzyme degradation of commercial CS.
Commercial CS was dissolved in enzyme buffer and 30µl of the enzyme was added. Digestion was measured
continuously by the change in absorbance at 232 nm on a spectrophotometer.
188
3.30 Assignment of unsaturated HS dissacharides from cockle GAG extracts
In order to examine the HS disaccharide compositions of crude cockle GAG extracts,
smples were digested with heparinases 1, 11 & 111 enzymes. The resulting oligosaccharides
were applied to a Pro-Pac PA-1 SAX-HPLC column (see materials and methods section for
details). The number of peaks generated from crude cockle GAG extracts was compared to
HS disaccharide standards obtained from complete digestion of commercial HS GAGs. The
results obtained from this analysis, revealed that the invertebrate glycosaminoglycan yields
mainly, the non- sulfated disaccharides ∆UA (1→4) GlcNAc (I) with retention time (Rt) 16
minutes (Table 6). Both N-sulfated ∆UA (1→4) GlcNS disaccharide and 6- O-sulfated ∆UA
(1→4) GlcNAc6S disaccharides were also detected (18 and 5% respectively).
It is notewhorthy, that the two unsaturated disaccharides (∆UA (1→4) GlcNS6S and
∆UA2S (1→4) GlcNS) peaks were also present in cockle HS but the percentage composition
of each was less than one. Additionally, the mono-sulfated ∆UA2S (1→4) GlcNAc, the rare
disulfated disaccharide (∆UA2S (1→4) GlcNAc6S) and the trisulfated disaccharide (∆UA2S
(1→4) GlcNS6S) were completely absent in crude cockle HS-GAG and this form the major
difference between the crude and the commercial GAG mixture.
Furthermore, to confirm whether cockle GAGs contain low sulfated HS-like
disaccharides, a portion of the crude extract was also digested with heparinise III enzyme and
the resulting oligosaccharides resolved by SAX-HPLC revealed that the main disaccharides
composition in cockle GAGs is non-sulfated ∆UA (1→4) GlcNAc disaccharide. Similarly,
both N-sulfated ∆UA (1→4) GlcNS and 6- O-sulfated ∆UA (1→4) GlcNAc6S disaccharides
peaks were also detected. However, the other three disaccharides (∆UA (1→4) GlcNS, ∆UA
(1→4) GlcNS6S and ∆UA2S (1→4) GlcNS) peaks were completely absent in cockle HS-like
189
GAGs, in contrast to what was observed for the commercial HS digested with heparinise III
(result not shown).
These results suggest that cockle mixture contain low sulfated HS-like GAGs and the
disaccharides composition analysis also suggests that this mollusc HS-like GAG contain non-
sulfated ∆UA (1→4) GlcNAc disaccharide as its main disaccharides.
190
Table 6: HS Disaccharides compositions from heparinase digest of cockle GAG extracts
HS disaccharides Cockle GAG mixtures
disaccharide compositions
(%)
Commercial HS-GAG
disaccharide compositions
(%)
∆UA (1→4) GlcNAc 75 55.00
∆UA (1→4) GlcNS 18 18.00
∆UA (1→4) GlcNAc6S 5.0 5.0
∆UA2S (1→4) GlcNAc Not detected 6.0
∆UA (1→4) GlcNS6S <1.0 2.0
∆UA2S (1→4) GlcNS <1.0 7.0
∆UA2S (1→4) GlcNAc6S Not detected <1.0
∆UA2S (1→4) GlcNS6S Not detected 6.0
The percentage compositions of each disaccharides peak was calculated using peak area
values obtained from SAX-HPLC software.
191
3.31 Gel Filtration analysis (TSK 2000PW) of heparinase degraded cockle GAG
extracts
A pilot study was conducted in order to ascertain the minimum amount of enzymes
and time required to digest completely 1mg commercial HS and 1mg of crude cockle GAGs.
Digestion was monitored by observing changes in the gel-filtration profile of the sample
(result not shown). The digestion appeared complete after additions of 30mU of Heparinase I,
II and III and incubation for a 48-hour period at 37 0C. Further addition of enzyme and
incubation for a further 24 hours caused degradation of the disaccharides into smaller units
(monosaccharide) (results not shown).
After 48 hours’ incubation of either crude or commercial HS GAGs with Heparinase
I, II and III enzymes, a 50 μl of the digested sample was applied to TSK 2000PW column and
the eluted profile was monitored at 232 nm for 180 minutes. The elution profiles obtained for
both comercial HS and crude cockle GAGs confirmed a complete digestion of both samples
as shown in Figure 3.30 (A-B). This result confirms the SAX-HPLC finding presented in the
previous section and the single broad peak obtained correspond to HS disaccharides.
192
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Elution time in minutes
dp2
dp2
dp6
dp8
dp4
a b
dp10
dp2
193
Figure 3.30: Analytical TSK2000PW gel-filtration profiles of HS/Heparin and crude
cockle GAGs after complete digestion with Heparinase I, II and III
enzymes
50 µg of the enzymes GAGs digest by the Heparinase I, II and III enzymes were chromatographed on a
TSK2000PW analytical gel-filtration column (30 x 0.75 cm) and the elution was monitored at 232 nm for 180
minutes. (A) Elution profile for commercial HS/Heparin standard digested in Heparinase I, II, and III. (B)
Elution profile for crude cockle GAGs digested in Heparinase I, II, and III. (C) Elution profile for HS/Heparin
digested in Heparinase I enzyme. Abbreviations: dp10
- octasaccharides: dp8- heptasaccharides: dp
6-
hexasaccharides: dp4- tetrasaccharides: dp
2- disaccharides.
3.32 Superose 12 size exclusion chromatography analysis of intact cockle extracts
GAG chains
Cockle GAG extracts were analysed for size using a superose 12 size exclusion column.
GAG content of the fractions collected from this column was determind by cellulose acetate
dot blotting assay. This showed that fractions 1-14 & 28-40 did not contain any GAGs
(Figure 3.31), however fractions 15-27 showed distinct binding of azure A stain to the
sulfated GAG components present in these fractions. The intensity of the stain is relatively
proportional to the concentrations of GAGs present in each fraction i.e. the more GAGs in the
fraction, the deeper the stain. Quatitative analysis of GAGs compositions in crude cockle
GAG extracts was determind by densitometry analysis; the result shows two major GAGs
containing peaks were eluted from the Superose 12 column. The larger molecular weight
species [fractions 15- 20 (A)] were eluted first, followed by the smaller polysaccharide
[fractions 21-27 (B)].
194
A
B
Figure 3.31: Superose 12 size exclusion chromatography and cellulose acetate dot
blotting result for crude cockle GAG mixture
(A) Cellulose acetate dot blotting assay result for crude cockle GAG mixture (B) Densitometry and scan
analysis of cellulose acetate dot blotting: each peak represents GAG with relative size based on their structural
composition and ionic contents (SO3 and COO-)
11 12 13 14 15 16 17 18 19 20
21 22 23 24 25 26 27 28 29 30
31 32 33 34 35 36 37 38 39 40
A B
195
3.33 PAGE analysis of crude cockle GAG extracts and commercial GAGs after
enzymatic depolymerisation.
The crude cockle GAG extracts and commercial GAGs treated separately with
heparinase (I, II, and III) and ABC lyase enzymes were analysed using PAGE. The results are
presented in Figure 3.32.
All intact GAG samples show slow moving and very diffuse and unresoved bands [(Figure
3.32 (2, 3, 5 and 8)], indicating a heterogeneous mixture of GAG chains. Conversely, all the
enzyme-treated samples demonstrated faster-moving bands; thus indicating shorter chain
oligosaccharides due to degredation of chains by the enzymes [(Figure 3.32 (1, 4, 6 and 7)].
These results confirmed the presence of both CS/DS-like and HS-like oligosaccharides in the
crude cockle GAG extracts.
196
Figure 3.32: PAGE analysis of enzymatic depolymerised GAGs.
All the commercial GAGs and crude cockle GAG mixture were incubated with heparinase (I,II, and III) and
ABC lyase enzymes separately for 48 hours and approximately 20 μl of the degraded sample was applied to
each lane. (1) Crude cockle GAG extracts digested with ABC lyase enzyme. (2) Intact crude cockle GAG
extracts. (3) Intact crude cockle GAG extracts. (4) Crude cockle GAG extracts digested with Heparinase I,II,
and III enzymes. (5) Intact HS commercial GAG (6) HS-GAG sample digested with Heparinase I, II, and III
enzymes. (7) CS GAG digested with ABC lyase enzyme. (8) Intact CS commercial GAG.
1 2 3 4 5 6 7 8
197
Section 3E
Characterisation of crude whelk
GAG mixtures
198
3.34 Assignment of unsaturated CS dissacharides for whelk GAG extract
Whelk GAG extracts was digested with the enzyme chondroitinase ABC lyase in
order to determine the presence of CS/DS-like GAGs. The digestions were monitored
spectrophotometrically at 232 nm until completion was observed (Figure 3.33A-C).
199
Figure 3.33: Kinetic of chondroitinase ABC enzyme degradation of GAGs
Commercial CS and whelk GAGs was each dissolved in enzyme buffer and 30µl of the enzyme was added to
each dissolved sample. Digestion was measured continuously by the change in absorbance at 232 nm on a
spectrophotometer. (A) Commercial CS in chondroitinase ABC enzyme (B) Crude whelk GAG in
chondroitinase ABC enzyme (C) Whelk fraction C in chondroitinase ABC enzyme.
A
B
C
200
The elution profile for crude whelk GAG extracts, compared with the reference
chromatogram, showed that the crude whelk GAG extracts contain both CS/DS-like
disaccharides (Table 7). The percentage composition of each disaccharide peak was
calculated and data recorded in table 4. The main disaccharides peaks, as resolved by SAX-
HPLC, are mono-sulfated disaccharide (ΔDi-6S) composed of ΔUA→3GalNAc (6S) and
(ΔDi-4S) composed of ΔUA→3GalNAc (4S). These two peaks compared favourably, by
retention time, with the commercial CS disaccharides peaks. However, there are other broad
peaks eluted along with the disaccharides, which may indicate partial digestions or resistance
of the polymer to chondroitinase ABC lyase.
201
Table 7: Disaccharides compositions of CS/DS-like glycans found in whelk GAG
extracts
Disaccharides Whelk GAG composition (
%)
Commercial CS
composition ( %)
Δ UA-GalNac Not detected Not detected
Δ UA-GalNac (6S) 55 73
Δ UA-GalNac (4S) 45 27
Δ UA (2S)-GalNac Not detected Not detected
Δ UA-GalNac (4S,6S) Not detected Not detected
Δ UA (2S)-GalNac (6S) Not detected Not detected
Δ UA2S-GalNac4S Not detected Not detected
The percentage compositions of each disaccharides peak was calculated using peak area
values obtained from SAX-HPLC software.
202
3.35: PAGE analysis of crude whelk GAG extracts and commercial GAGs after
enzymatic depolymerisation.
The crude whelk GAG extracts and commercial GAGs were treated separately with
heparinases I, II and III and with ABC lyase enzymes and analysed using PAGE. The results
are presented in Figure 3.34.
All the intact GAG samples show a very diffuse bimolecular weight band [(Figure 3.34 (2, 3,
5 and 8)], indicating a long linear polymer chain with hetergenous populations. Conversely,
all the enzyme treated samples showed faster moving less intensely stained bands indicating
shorter chain oligosaccharides as products of enzymatic digestion, these differences can be
used to determine the specific presence of GAG subfamilies based on the enzymatic
specificities of the enzymes [Figure 3.34 (1,4,6 and 7)].
These results confirmed the presence of both CS/DS-like and HS-like
oligosaccharides in the crude whelk GAG mixtures.
203
Figure 3.34: PAGE analysis of enzymatic depolymerised GAGs.
All the commercial GAGs and crude whelk GAG extracts were incubated with heparinase (I, II, and III) and
ABC lyase enzymes separately for 48 hours and approximately 20 μl of the degraded sample was applied to
each lane. (1) Crude whelk GAG extracts digested with Heparinase I, II,and III enzymes. (2) Intact crude whelk
GAG extracts. (3) Intact HS commercial GAG. (4) HS commercial GAG digested with Heparinase I,II, and III
enzymes. (5) Intact whelk GAG extracts (6) Whelk GAG extracts mixture digested with ABC lyase enzyme. (7)
CS commercial GAG digested with ABC lyase enzyme. (8) Intact CS commercial GAG.
1 2 3 4 5 6 7 8
204
3.36 Superose-12 size exclusion chromatography of crude whelk GAG Extracts.
The results obtained show that crude whelk GAG extracts contain five main peaks
with varying sizes, by UV monitoring and GAG binding dot blot assay.The void volume of
the column (V0) was calculated as being at fraction 14, as shown in Figure 3.35, with
fractions (15-32) contains varying concentrations of GAGs within the five peaks eluted. The
qualitative analyses of the five GAG peaks were performed using densiometry of the stained
dot blot. Each peak represents different populations of GAG chains eluting according to their
sizes. Fractions 15-17 being the largest GAG component eluted and fractions 30-32 being the
smallest.
205
B
Figure 3.35: Superose 12 size exclusion chromatography and cellulose acetate dot
blotting assay of crude whelk GAG extract.
(A) Cellulose acetate dot blotting assay result for crude whelk GAG mixture (B) Densitometry and scan analysis
of cellulose acetate dot blotting.
10 11 12 13 14 15 16 17 18
19 20 21 22 23 24 25 26 27
28 29 30 31 32 33 34 35 36
A B
C
D
E
206
SECTION 3F
Characterisation of purified whelk
GAG peaks derived by ion exchange
chromatography
207
3.37 Assignment of unsaturated CS dissacharides from purified whelk GAG fractions
In order to ascertain which of the whelk GAG peaks obtained from the ion exchange
column contain CS/DS-like GAGs, samples were digested with chondroitinase-ABC lyase.
The resulting oligosaccharides products were analysed by SAX-HPLC. Only two fractions (B
and C) from the ion exchange column (Table 8) were sensitive to depolymerisation by
chondroitinase ABC lyase, the other three peaks (A, E & F) were resistant to the action of
this enzyme. The depolymerised whelk GAG peaks B and C produced two major peaks
which were identified as Δ UA-GalNac6S and ΔUA-GalNac4S. The oligosaccharides peaks
were identified by comparing their elution positions with those of standard oligosaccharides
obtained from commercial CS GAGs.
The SAX-HPLC separation of the unsaturated oligoccharides produced by the action
of chondroitinase-ABC on purified whelk fraction B produced three major disaccharide
peaks, assigned to unsaturated non-sulfated Δ UA-GalNac (di-0S), mono-sulfated Δ UA-
GalNac6S (Di-6S) and ΔUA-GalNac4S (DI-4S). From the peak areas, it could be calculated
that these three disaccharides contain 55% Δ UA-GalNac, 35% Δ UA-GalNac6S and 10 %
ΔUA-GalNac4S of the total disaccharide composition (Table 8). Other unidentified peaks
were also eluted with the oligosaccharides which may be an indication of contamination or
imcomplete digestion of the polymer.
Simlarly, SAX-HPLC result of depolymerised peak C demonstrated two major
disaccharides peaks with similar elution profiles to the commercial CS disaccharides (Table
5). The first peak was assigned the mono-sulfated disaccharide Δ UA-GalNac6S (ΔDi6S).
Also from the peak areas, it could be calculated that these two disaccharides contain 22% Δ
208
UA-GalNac (6S) and 78 % Δ UA-GalNac (4S). Other unidentified peaks were also eluted
along with the disaccharides which may suggest contamination or resistance to
chondroitinase-ABC enzyme.
Fractions A, F and the biologically active fraction E were found to be resistant to chondroitin
ABC lyase treatment and did not produce any degredation peaks. Further investigation of the
biologically active fraction E was obviously required in order to confirm the nature of the
GAG components that it contains.
209
Table 8: Disaccharides compositions of CS/DS-like GAGs present in ion-exchange
purified whelk peaks B and C
Disaccharides Whelk fraction B
disaccharide
composition ( %)
Whelk fraction C
disaccharide
composition (%)
Commercial CS
disaccharide
composition ( %)
Δ UA-GalNac 55 Not detected Not detected
Δ UA-GalNac (6S) 35 22 23
Δ UA-GalNac (4S) 10 78 77
Δ UA (2S)-GalNac Not detected Not detected Not detected
Δ UA-GalNac (4S,6S) Not detected Not detected Not detected
The percentage composition of each disaccharides peak was calculated using peak area
values obtained from SAX-HPLC software.
210
3.38 Heparinase I-III enzymatic treatments and disaccharide analysis by SAX-HPLC
of the active whelk fraction E
To further elucidate the HS-like disaccharides in ion-exchange purified whelk GAG peak
(fraction E), the pooled biologically active fraction E was digested with Heparinase I, II, and
III enzymes. The resulting oligosaccharides were resolved by SAX-HPLC and showed six
confirmed HS disaccharide peaks with some minor contamination from other unidentified
peaks. The major disaccharides peak from the heparinase digested fraction E was assigned to
non- sulfated HS disaccharide ∆UA- GlcNAc, which comprised 60 % of the total
disaccharide composition of fraction E (Table 9). The N-sulfated disaccharide ∆UA -GlcNS
was also present with a percentage composition of 29%. The 6- O-sulfated ∆UA -GlcNAc6S
disaccharide has a percentage composition of 2% of the total disaccharides composition. The
forth peak was assigned to the unsaturated ∆UA-GlcNS (6S) disaccharide with a percentage
composition of 7 %. The fifth peak was assigned to the rare di-sulfated ∆UA (2S)-GlcNAc6S
disaccharide with a very low composition of less than 1%. The tri-sulfated disaccharides
∆UA (2S) (1→4) GlcNS (6S) was also present in this polysaccharide but the percentage
composition was very low (1%). Interestingly, the 2-O-sulfated ∆UA (2S)-GlcNAc and ∆UA
(2S)-GlcNS disaccharides were completely absent from this polymer and this form the major
difference between this novel and the commercial HSGAGs disaccharides. However the
disaccharide analysis couldn’t rule out the presence of disaccharides not normally seen in HS
that might account for the different activities observed with Whelk derived GAGs and
commercial HS.
Fraction E was also digested with heparinases I, II, and III individually, to identify the
specific enzyme or enzymes responsible for the depolymerisation of whelk fraction E.
Enzymatic activities were monitored by following the increase in UV absorbance at 232 nm
211
with time and the resulting oligosaccharide were applied to SAX-HPLC column and resolved
using a NaCl gradient. Heparinase I and II showed limited ability to degrade the fraction E
GAGs. In contrast, heparinise III demonstrated significant activity against this polysaccharide
(Table 10). This result suggests that whelk fraction E contains a significant proportion of low
sulfated HS-like GAG chains.
212
Table 9: Disaccharides compositions of HS-like GAGs found in purified whelk fraction
E.
HS disaccharides Whelk fraction E
disaccharide composition
(%)
Commercial HS
disaccharide compositions
(%)
∆UA (1→4) GlcNAc 60 55.00
∆UA (1→4) GlcNS 29 18.00
∆UA (1→4) GlcNAc6S 2 5.0
∆UA2S (1→4) GlcNAc Not detected 6.0
∆UA (1→4) GlcNS6S 7 2.0
∆UA2S (1→4) GlcNS Not detected 7.0
∆UA2S (1→4) GlcNAc6S <1 <1.0
∆UA2S (1→4) GlcNS6S 1 6.0
The percentage composition of each disaccharides peak was calculated using peak area
values obtained from SAX-HPLC software.
213
Table 10: Disaccharides compositions of HS-like GAGs found in purified whelk fraction
E depolymerised by heparinase III lyase.
HS disaccharides Whelk fraction E
disaccharide composition
(%)
Commercial HS
disaccharide compositions
(%)
∆UA (1→4) GlcNAc 75.00 59.00
∆UA (1→4) GlcNS 16.00 22.00
∆UA (1→4) GlcNAc6S 1.00 4.00
∆UA2S (1→4) GlcNAc Not detected 7.00
∆UA (1→4) GlcNS6S 8.00 2.00
∆UA2S (1→4) GlcNS Not detected 6.00
∆UA2S (1→4) GlcNAc6S Not detected Not detected
∆UA2S (1→4) GlcNS6S Not detected Not detected
214
3.39 HPLC Gel Filtration analysis of whelk fraction E after heparinase degradation
The digestion of the purified whelk fraction E was monitored through changes in the
gel-filtration profile of the sample (result not shown). The digestions appeared complete after
additions of 30mU of Heparinase I, II and III, followed by continuous incubation for 48 hour
period at 37 0C. After 48 hours’ incubation of purified whelk fraction E or HS/heparin GAG
with heparinase I, II and III enzymes, a 50μl of the digested sample was applied to TSK
2000PW column and the eluted profile was monitored at 232 nm for 180 minutes. The elution
profiles obtained for both HS/Heparin and purified whelk fraction E confirm complete
digestion of both samples as shown in Figure 3.36 (A-B). This result confirms the SAX-
HPLC result described in the previous section and the single broad peak obtained
corresponds to HS disaccharides (dp2).
However, heparin digested with Heparinase I enzyme for 48 hours shows a number of
oligosaccharide peaks in addition to the usual disaccharide peak; an indication of incomplete
degradation of the commercial GAGs. The peaks corresponding to the various
oligosaccharides are also labelled appropriately in Figure 3.36 (C). Both SAX-HPLC and
TSK gel-filtration results confirmed the presence of HS-like disaccharides in the purified
fraction E.
215
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dp8
dp2
dp6
dp4
dp10
dp2
dp2
216
Figure 3.36: Analytical TSK2000PW gel-filtration profiles of HS/heparin and purified
whelk fraction E after complete digestion with Heparinase I, II and III enzymes.
50 µg of the enzymes GAGs digest by the Heparinase I,II and III enzymes were chromatographed on a
TSK2000PW analytical gel-filtration column (30 x 0.75 cm) and the elution was monitored at 232 nm for 180
minutes. (A) Elution profile for commercial HS/Heparin standard digested in Heparinase I,II, and III. (B)
Elution profile for purified whelk fraction E digested in Heparinase I, II, and III. (C) Elution profile for
HS/Heparin digested in Heparinase I enzyme.
Abbreviations: dp10
- octasaccharides: dp8- heptasaccharides: dp
6- hexasaccharides: dp
4- tetrasaccharides: dp
2-
disaccharides.
3.40 PAGE analysis of purified whelk fractions and commercial GAGs after
enzymatic depolymerisation.
The purified whelk GAG extracts and commercial GAGs were digested individually
and with a mixture of Heparinases I, II, and III enzymes. Similarly, these polysaccharide
fractions were also digested individually with ABC chondroitinase enzyme. The resulting
oligosaccharides from each enzyme digestion were analysed using PAGE (Figure 3.37).
All the intact GAG samples show a very intense and diffuse banding pattern [(Figure 3.37 (2,
3, 5 and 8)] indicating a heterogeneous mixture of polymer chains, a unique characteristic of
GAGs polymers.
Conversely, all the sensitive enzyme-treated samples show less intensely staining
bands and faster mobilities, suggesting breakdown into shorter chain oligosaccharides
[(Figure 3.37 (1,4,6 and 7)].
This result confirmed the presence of both CS/DS and HS-like oligosaccharides in the crude
and purified whelk GAG mixtures.
217
Figure 3.37: PAGE analyses of enzymatic depolymerised whelk derived and
commercial GAGs.
All the commercial GAGs and crude purified whelk fractions were incubated with heparinase (I,II, and III) and
ABC lyase enzymes separately for 48 hours.(1) Intact fraction C dissolved in enzyme buffer. (2) Purified
fraction C digested with chondroitinase-ABC lyase. (3) CS commercial GAG digested with chondroitinase-ABC
lyase.intact HS commercial GAG. (4) Intact CS commercial GAG dissolved in enzyme buffer (5) Intact purified
whelk fraction E dissolved in enzyme buffer. (6) Purified fraction E digested with Heparinase I, II and III. (7)
Intact commercial HS dissolved in enzyme buffer. (8) HS commercial GAG digested with Heparinase I,II, and
III enzymes.
1 2 3 4 5 6 7 8
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3.41 Superose-12 size exclusion chromatography of purified whelk fraction E
The results obtained from these analyses revealed that purified whelk fraction E
contain sulfated GAGs, as illustrated in Figure 3.38 since azure A binds to GAGs in this
fraction.The GAG content/overall sulfate content in each fraction is proportional to the
intensity of staining. Scanning densitometry analysis of the cellulose acetate dot blotting
assay shows that fraction E contains one major and high molecular weigh GAG componant,
this corresponds to the largest peak seen in the superpose-12 seperation of the un-fractionated
crude GAG extract (Figure 3.35). It also contains a minor peak corresponding to one of the
smaller GAGs eluted from initial crude whelk GAG mixture.
219
A
B
Figure 3.38 Superose-12 size exclusion chromatography and cellulose acetate dot
blotting assay for purified fraction E GAG mixtures
(A) Cellulose acetate dot blotting assay result for purified fraction E (B) Scanning densitometry analysis of
cellulose acetate dot blots: each peak represents GAG with relative size based on their structural composition
and ionic contents (SO3 and COO-).
A
B
220
Section 4
Discussion
221
4.1 Outline of the major findings
The results of this study provide significant insight into the pharmacological properties of
whelk and cockle derived GAGs in different cancer cells, including breast, cervical and
leukaemia cell lines. A summary of the main findings are indicated below:
Whelk GAGs inhibit the growth of negative eastrogen receptor (ER-ve
) breast cancer
cell in vitro (MDA468 and MDANQ01)
Whelk GAGs also inhibit the proliferation of cervical cancer cell (HeLa) in vitro
They also inhibits the growth of both erythroleukaemia (K562) and lymphoblastic
(MOLT-4) leukaemia cell in vitro
Whelk GAGs cause cell cycle arrests in both leukaemia and breast cancer cell
Whelk GAGs induce apoptosis in both cervical and leukaemia cell
Whelk GAGs contain both CS/DS and HS-like GAGs
Fraction E obtained by ion-exchange chromatography of whelk GAG extracts showed
selective anti-cancer activity against breast cancer cell lines.
Fraction E caused cell cycle arrest and initiated apoptosis in breast cancer cell lines
Cockle derived GAGs showed selective anti-cancer activity against both
erytholeukaemia and lymphoblastic leukaemia cells
Cockle GAGs brought about cell cycle arrest on lymphoblastic leukaemia cells
Cockle GAGs induced apoptosis on lymphoblastic leukemia cells
222
Cockle GAG extracts contained both HS and CS/DS-like GAGs
223
4.2 Selective anti-cancer activity of cockle GAGs against leukemia cell lines
Previous studies have revealed the anti-cancer activities of some GAG-like
compounds, for example, low molecular weight heparin, HS mimetics and some modified
CS/DS compounds (Afratis et al 2012 : Babara et al 2012 : Neha et al 2010 : Mellor et al
2007). No studies have linked therapeutic activity of mollusc derived GAGs to anti-cancer
activity in breast and leukemic cancer cells. GAG extracts isolated from cockle molluscs had
a significant growth inhibitory effect (p<0.001) on erythrocytic leukemic cells (K562) and
lymphoblastic leukemic cell (MOLT-4) (fig.3.3A and 3.4A). The recorded IC50 for the two
cell lines were 16 (MOLT-4 cell line) and 50 (K562 cell line) µg/ml respectively. According
to the standard criteria set by the National Cancer Institute (Chen et al, 1988; Geran et al,
1972), crude natural product extracts possessing an IC50 of less than 20 μg/ml are considered
active against appropriate cancer cell lines.
Cockle GAGs extracts revealed a recorded IC50 of less than 20 μg/ml in MOLT-4 cell
proliferation assay and this according to the National Cancer Institute categorise it as an
active anti-leukemic cancer drug. Interstingly, this GAG mixture was non-toxic to a normal
fibroblast cell line (3T3); a cell line that is frequently used as the model for the cytotoxicity
testing in normal cells. Similarly, high concentration of cockle GAG extracts did not show
any effect on cell proliferation of MDA468 and MDANQ01 breast cancer cells (fig.3.1A &
B). In this regard, the cytotoxicity of this novel GAG was highly selective against K562 and
MOLT-4 leukemic cell type and non-toxic to normal cells. It would be interesting to
determine the exact biochemical nature of this selectivity and if time had allowed a LC
MS/MS proteomic and pathway analysis examination would have been attempted before and
after treatment with the crude GAG extracts.
224
4.3 Evidence of broader and stronger anti-cancer activity of whelk GAGs extracts
Globally, breast cancer is currently one of the leading causes of death and the most
commonly diagnosed cancer in women aged below 39 years. Among women aged 35-39 in
the UK, around 1,350 cases of breast cancer are diagnosed each year (Breast cancer 1975-
2010). Estrogen receptor negative (ER-ve
) breast cancers are tumours with a distinct natural
history, treatment response, and prognostic profile (Wang and Lin 2008). ER-ve
breast cancers
make up 25%–30% of all breast cancers, and their clinical course tends to be more aggressive
than that of estrogen receptor positive (ER+ve
) breast cancers (Wang and Lin 2008). Patients
with ER-ve
breast cancer generally have shorter disease-free survival and overall survival
times (Wang and Lin 2008). Most patients with ER-ve
tumours do not benefit from anti-
hormonal therapy, and are also disadvantaged because of the resistance issues associated with
many anti-cancer therapies (Wang and Lin 2008). Conventional breast cancer treatment
involves surgery that may be coupled with radiation, chemotherapy and systemic adjuvant
therapy (Koo et al, 2008).
The approach of modulating tumour progression with drugs that inhibit growth of
tumours is one of the new concepts in adjuvant chemotherapy when used alone or in
combination with classic anti-tumour drugs (Basappa et al, 2012). Currently, there is great
interest in the search for new anti-cancer drugs that can improve patient responses to cancer
treatment and reduce the number of deaths, while minimizing the side effects. Certain types
of GAG chain have been reported to be potentially useful in cancer therapy and are predicted
to have minimal side effects (Basappa et al, 2012).
Our data, which shows selective activity amongst tumour cell lines and normal tissue,
would support this idea and the therapeutic use of these GAGs now seems like an even more
attractive proposition.
225
The presence of GAGs in both vertebrates and invertebrates has been attributed to
many physiological and biological roles including carcinogenesis and angiogenesis through
its interaction with some growth factors and their receptors (Gomes et al, 2010). Yamada and
others have reported the isolation of all groups of GAGs including sulfated and non-sulfated
from many animals including molluscs (Yamada et al, 2007: Nader et al, 1983: Cassaro and
Dietrich, 1977).
The whelk GAG extracts demonstrated unique anti-cancer activity against many
cancer cells including Estrogen receptor (ER)-negative breast cancer in vitro. It is an
extremely important observation for possible intervention in the hard to treat cancers. In
contrast to the observed selective anti-cancer activity of cockle GAG extracts against certain
cancer cells, whelk GAG extracts, was cytotoxic to all cancer cell lines tested in this work.
This GAG extracts demonstrated significant (p<0.001) growth inhibitory effects on both
MDA468 and MDANQ01 breast cancer cell with recorded IC50 70.96 and 25.14 µg/ml
respectively. The growth inhibitory effect of this novel GAG on the two breast cancer cell
lines tested were shown to be dose-dependent and MDANQ01was more sensitive to the
GAG’s treatment than MDA468.
These results suggests a possible synergy between the reductase enzyme that is
present in MDANQ01 and whelk GAG mixture which may have made the cell line more
susceptible to growth inhibitory effects of whelk GAG mixture. It is very likely that other
gene difference play a role in the observed selectivity and only a detailed
proteomic/transcriptomics and pathway analysis may resolve this. The growth inhibitory
activity of whelk GAG mixture was comparable to the effect of cisplatin anti-cancer drug on
the two cancer cell lines (Figure 3.9A and 3.10A).
226
However, the results obtained earlier for similar GAGs extracted from another
shellfish (cockle GAG) did not show any inhibitory effect on the proliferation of these breast
cancer cells; thereby suggesting that the inhibitory effect may be a unique fine structural
feature of the GAGs derived from whelks. In addition, the non-toxic activity of all other
commercial GAGs (HS/Heparin and CS/DS) tested along side whelk GAG mixtures on the
two breast cancer cell lines suggest that the whelk GAG contains some unique structural
features not seen in the commercial GAG samples. These structural features may be a unique
pharmacological feature that makes whelk derived GAGs a potential candidate as the basis
for a future anti-cancer drug.
Furthermore, whelk GAG Extracts were also cytotoxic to erythrocytic (K562) and
lymphoblastic (MOLT-4) leukemic cells (Figure 3.11A&B). The cytotoxic activity of whelk
GAG mixture was more pronounced on both cervical (Hela) and erythrocytic leukemic cells
with recorded IC50 of 10.47 and 12.57 µg/ml respectively (Figure 3.11 and 3.12). However, a
higher IC50 of 49.11 µg/ml was recorded for lymphoblastic leukemia cell but this GAG
extract did not show any noticeable cytotoxic activity against normal fibroblast cell (3T3), an
indication of selective activity against cancer cell growth. Indeed the differences in IC50
values for the five different cancer cell lines suggests that the whelk GAG mixtures could be
selective to certain cell types and this selectivity may well be important in targeting the
effects of these molecules towards tumour cells.
Additionally, in breast cancer, changes in GAG and proteoglycan expression on the
cell surface and in the ECM allow tumour cells to proliferate, gain the ability to invade
surrounding tissues, metastasize to distant organs and induce angiogenesis (Koo et al, 2008).
Therefore, a novel exogenous GAG (like the whelk GAG extracts) with unique structural
composition may modulate this effect in various ways (see later discussion), which may
ultimately leads to growth inhibition observed in this study. The whelk GAG extracts may act
227
in several ways: by activating (agonists) or inactivating (antagonists) protein-based receptors,
competing with endogenous GAGs and/or inhibiting GAG biosynthesis etc. (Ghandi and
Mancera, 2010).
This result is also consistent with the findings of Linhardt and others who have
identified some new classes of GAG chain-based molecules (neoglycans, low molecular
weight heparin, ultra low molecular weight heparin, HS mimicking compound and heparin
mimicking compound) with anticancer activity ( Lindhardt 2011: Xu et al 2011:Zhou et al
2011) . Whelk GAG extracts show comparative anti-cancer activities to this class of GAG
chain-based molecules with similar IC50. However, native CS and unfractionated heparin did
not inhibit cell death in all the cancer cells tested along with the GAG chain drugs:
commercial GAGs likewise did not have any growth inhibitory effect on any of the cancer
cells tested in this study (Afratis et al 2012: Linhardt and Liu 2012: Borsig et al 2011: Neha
et al 2010: Pumphrey et al 2002)
4.4 Selective anti-cancer activity of whelk bioactive fraction E against breast cancer
cell.
It has been reported previously that understanding the fine structure and specific
biological roles of GAGs may lead to the development of novel therapeutic approaches
(Afratis et al, 2012). In order to study the fine structure of the whelk GAG mixtures, the
crude extract was purified by ion-exchange chromatography and the resulting fractions were
tested on some cancer cell lines (Figure 3.23 and 3.24). All the fractions eluted were non-
toxic to breast cancer cell except fraction E. Fraction E was found to be cytotoxic to both
MDA468 and MDANQ01 with recorded IC50 value of 45.98 and 41.89µg/ml respectively.
The cytotoxic effect of fraction E on both cancer cell lines was dose-dependent and similar to
228
the crude extracts. In contrast to the crude extract, fraction E was non-toxic to other cancer
cell lines such as HeLa, K562, MOLT-4 and normal fibroblast (3T3) cell.
These results suggests that this fraction E was selective against breast cancer cells,
mirroring that results seen for the original crude whelk GAG mixtures and may possess a
unique structure that inhibits the growth of breast cancer cell lines tested in this study (see
later discussion). The results with fraction E suggests that this fraction is the bioactive
component responsible for the anti-cancer activity of whelk GAG extracts, at least those seen
with the breast cancer cell lines. Further understanding the exact structural features seen in
this particular fraction may open a new therapeutic approach to cancer therapy.
4.5 Molecular mechanism of action of cockle GAG extracts on leukaemia cell lines
Recently, cell cycle analysis has been used to identify a molecular target for new anti-
cancer drugs (Basappa et al, 2012: Dawson et al, 2008: Marks 2007 and Tiligada et al, 2002).
Cellular proliferation is mediated primarily by cell cycle which consists of four distinct
sequential phases (G0/G1, S, G2, M).They are controlled by cellular signalling regulatory
mechanisms involving a family of proteins that have variable level of expression according to
the stage of the cell cycle (van den Heuvel 2005: Jack and Weinberg, 1996).
Perturbations in cell cycle regulation are reported as one of the most common features
of the transformed cell (Weinstein, 1996), which could be associated with gain of function for
uncontrolled growth due to enhanced expression of growth-factor-receptor autocrine loop
(Earp et al, 1995). Several therapeutic agents including some anti-cancer drugs, such as
DNA-damaging drugs, microtubule inhibitors, anti-metabolites, and topoisomerase inhibitors,
take advantage of disruption in normal cell cycle regulation to target checkpoint controls and
ultimately induce growth arrest or apoptosis of tumourogenic cells.
229
Leukemia cell are known to be very sensitive to any chemotherapeutic agents/drug
that either disrupt the cell cycle or cause apoptosis (Askoy et al 2008). Some of these
chemotherapeutic agents cause leukemia cell death through usual DNA disruption, while
others cause cell death by programmed cell death (apoptosis); a key player in the balance
between cell replication and cell death (Feng et al 2007). Many chemotherapeutic agents are
effective on the cells that are in the S phase of the cell cycle (Askoy et al 2008). However,
other chemotherapeutic agents such as artemisinin mainly arrests the cell cycle in the G1
phase, while paclitaxel and lycorine were shown to arrest the cell cycle in the G2/M phase
and induce apoptosis by increasing the activation of caspase-8, caspase-9, or caspase-3
(Pezuto et al 1997). Similarly, an increase in the percentage of cells in the G2/M phase upon
treatment with sulforaphane was observed in HT29 human colon cancer cells as well as in
Jurkat T-leukemia (Singh et al 2004). Cisplatin also cause cell cycle arrest at both the G1/S
and G2/M checkpoints (Roberts and Thompson, 1979).
In the present study, cockle GAG extracts caused time-dependent disruption in
lymphoblastic leukaemia cell cycle regulations, resulting in G1 and G2/M-phase arrest with a
concomitant marked reduction of cells at S-phase. This result is consistent with the cell cycle
arrest cause by many other chemotherapeutic agents listed above which is primarily cause by
the accumulation of the chemotherapeutic agent. The ultimate effects might mediate DNA
strand breaks, which can cause the failure of DNA repair and subsequent arrest of the cell
cycle during the G1 and G2/M-phase. This result is also similar to the actions of other
chemotherapeutic agents which commonly intervene at multiple points in the cell cycle.
These drugs have been reported to have diverse mechanisms of action and exhibit
specificity in terms of the stage of the cell cycle in which they have activity (Johnson and
Walker, 1999). This type of checkpoint arrest (G1 and G2/M) is common to some DNA
damage anti-cancer drugs like cisplatin and is one of the most established chemotherapeutic
230
approaches in cancer treatment (Roberts and Thompson, 1979). Zhan et al.reported the
mechanisms of actions of cisplatin cell cycle arrest at G1 phase is mediated by p53, which
induces an increase in p21, resulting in inhibition of cyclin/cdk2 and cyclin/cdk4 complexes
and hypophosphorylation of Rb (Zhan et al, 1993).The G2/M checkpoint induced by DNA
damage can occur by either p53-dependent or –independent mechanisms (Zhan et al, 1993).
Both p21 and phosphorylation of cdk1 is required for entry into M and can participate in the
DNA damage G2/M checkpoint.
Fan and his co-worker also reported that tumour cells in which p53 is inactive can
bypass the G1/S checkpoint and exhibit increased sensitivity to DNA-damaging agents such
as cisplatin (Fan et al, 1997) as a result of failure to arrest and repair their damaged DNA.
These researches indicated that chemotherapeutic agent causes cell cycle arrest at both G1
and G2/M phase of the cell cycle similar to what was observed in the present study.
Therefore the G1 and G2/M cell cycle arrest cause by cockle GAG mixture on leukemia
cell may predictably has a similar mechanism of actions described by Zhan and Fan above.
Unfortunately, the cell cycle regulators (cyclins and cdk’s) that control G1 and G2/M
check points were not done during this project work and this may perhaps provide a better
explanation for the mechanism of cell cycle arrest caused by cockle GAG extracts. This
finding indicates that the cell growth inhibitory effect of cockle GAG extracts on leukaemia
cells is due, in part, to its cell cycle arrest. The mechanism underlying the cell cycle arrest
effect of cockle GAG mixtures remains unclear and this can easily be resolved by
investigating the cell cycle regulators that control the transition of cell at G1, G1/S (CDK2 ,
CDK4, cyclin E and D and CDKI’s) and G2/M (CDK1, cyclin A and B) phase using western
blotting analysis.
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4.6 Molecular mechanism of action of whelk GAG extracts on breast cancer cell
The perturbation of normal cell cycle controls, which is the hallmark of cancer,
provides numerous opportunities for targeting checkpoint controls to develop new therapeutic
strategies for this disease. Such strategies include induction of checkpoint arrest and arrest of
proliferating cells at various stages of the cell cycle, which may sensitize them to treatment
with other therapeutic agents such as radiation, and targeting of therapies towards specific
regulatory components of the cell cycle (Johnson and Walker 1999).
Matsui et al reported S-phase arrest caused by methotrexate and 5-fluorouracil, a
known DNA-damaging agent that inhibit DNA synthesis (Matsui et al, 1996). Lowel et al
also reported that tumour cells in which p53 is inactive, DNA damage induced by these drugs
goes undetected, and cells progress to G2 and subsequently undergo apoptosis (Lowel et al,
1993). Heparin GAG has shown antihypertensive, anti-inflammatory, anticoagulant in
different human cells including vascular smooth muscle cells (VSMC) (Leverand Page 2002).
Castellot and other groups demonstrated the antiproliferative activity of heparin on VSMC,
hepatoma and ovarian epithelial cell (Patel et al 2002: Fedarko et al 1989: Castllot et al
1985). It is generally accepted that heparin and heparin like GAGs including HS biological
activities is linked to their structure (SAR). However, Wright and other research groups
suggested the antiproliferative effect of heparin on VSMC was due to its ability to bind
VSMC surface receptor, accumulation within the cell and cell cycle arrest at both G0/G1 and
S phase (Reily et al 1996: Wright et al 1985). Scarffe et al, similarly reported an increase in
the percentage of cells in the G2/M phase upon treatment with sulforaphane in HT29 human
colon cancer cells as well as in Jurkat T-leukemia (Scarffe et al 1980).
Askoy et al in his recent in vitro work reported antiproliferative effect of heparin on
lymphoblast. They demonstrated that heparin induces cell cycle arrest of lymphoblast at both
232
G2/M and S phase in a dose and time dependent manner. Hence, suggested that the
antiproliferative effect of heparin on lymphoblast was mediated by cell cycle arrest at both
G2M and S phases, and the prolonged effect of the cell cycle arrest could play a role in cell
progression and proliferation (Aksoy et al 2008). These researches indicated that
chemotherapeutic agents including heparin GAG elicit their antiproliferative effect partly by
inducing cell cycle arrests at different stages of the cancer cell cycle. It is also shown that
heparin GAG elicit its antiproliferative activity by binding to its receptor on the cell surface;
accumulating within the cells and cell cycle arrests at different phases of the cell cycle.
In the present study, Whelk GAG extracts and the purified fraction E caused
consistent perturbation in breast cancer cell cycle control, which ultimately resulted into cell
cycle arrest at S and G2/M-phase. S-phase arrest is suggestive of cell inability to replicate,
which could abrogate the progression of cell cycle to the mitotic stage, the penultimate event
in the cell cycle. This GAG extracts and it’s purified fraction E induces cell cycle arrest of
both MDANQ01 and MDA468 breast cancer in a dose and time dependent manner (Figure
3.15-16 and 3.26&27). This result is consistent with the work of Aksoy et al on heparin GAG
cell cycle arrest on lymphoblast.
Heparin is a well established GAG that is structurally similar to HS and both crude
whelk and purified fraction E is a novel HS-like GAGs isolated from shellfish. The
comparative effect of heparin, crude whelk and purified fraction E GAGs on cell cycle arrests
may be structurally originated, however, it is difficult to conclude on this note unless a
comprehensive structural elucidation of the crude and purified fraction E is done.
Additionally, this result suggest that antiproliferative effects of both crude whelk and purified
fraction E GAG was mediated by cell cycle arrest at both S and G2/M phase and the
233
accumulative effect of the cell cycle arrests could play a role in the cell cycle progression and
cell proliferation.
4.7 Cockle GAG mixture inhibit proliferation of MOLT-4 leukaemia cell partly by
apoptosis
Apoptosis is another familiar molecular target for new anti-cancer drugs. Apoptosis
detection is of great importance in cancer research because the balance between cell
proliferation and apoptosis shifts towards cell proliferation in cancer cell lines. Cancer results
from the imbalance between cell proliferation and apoptosis (Wesselborg et al 1999).
Therefore there is an active search for the most efficient and safe anti-cancer treatments that
induce apoptosis in immortal cancer cells (Coppola et al, 2008).
Cockle GAG extracts only induced marginal early apoptotic effect on MOLT-4
leukaemia cell as shown in Figure 3.8. The apoptotic effect of cockle GAG extracts was
noticeable between 24 and 48 hours post incubation. Apoptosis plays a major protective
mechanism against cancer (Zhou et al 2004) and this result shows that cockle GAG extract
can induce apoptosis on MOLT-4 cells. This finding is consistent with the apoptotic effects
seen with chemically modified GAG chains and heparin on lymphoblast and other carcinoma
as described by Erduran and other research groups (Erduran et al 2007: Erduran et al 2004:
Pumphrey et al 2002: Li et al 2001: Erduran et al 1999: Manaster et al 1996). Manaster and
other research groups have earlier reported the apoptotic effect of heparin on various human
cells including peripheral blood neutrophils, lymphoblasts and mononuclear cells. They also
suggested that heparin apoptotic effect of lymphoblasts was via an extrinsic pathway of
apoptosis (Erduran et al 2007: Eduron et al 2004: Erduron et al 1999: Manaster et al 1996).
Pezuto et al also reported the apoptotic effect of paclitaxel and lycorine, (known
234
chemotherapeutic agents) and they demonstrated that the antiapoptotic effect of these drugs
were due to increase activation of caspace-3, 8 and 9 (Pezuto et al 1997). Erduran et al in
their work demonstrated that low dose of heparin (20 U/mL) causes apoptosis in the
lymphoblast and this low concentration also cause a high expression of Fas and a low
expression of Bcl protein-2 in the lymphoblast (Erduran et al 2004). This was contrary to the
in vitro work of Manaster and coworkers who reported apoptotic effect of heparin at very
high concentrations (50-200 U/mL) (Manaster et al 1996). In another recent in vitro study,
caspace 3 and 8 activation levels were investigated and it was shown that heparin induce
apoptosis of the lymphoblasts and activation of caspase-3 and -8 (Eduran et al., 2007)
Li et al in their work reported that heparin induce apoptosis in human nasopharyngeal
carcinoma cell (CNE2) and demonstrated the apoptotic effect of heparin on this cell may be
probably regulated by increased expression of c-myc and the rates of bax/ bcl-2. They
suggested heparin may function as an inducer of apoptosis in carcinoma cells (Li et al 2001).
These researches indicated that low-dose heparin caused significant levels of apoptosis of
lymphoblasts, and apoptosis was found to increase with increased heparin levels.
It is thus suggested that the growth inhibitory effect of cockle GAG extracts on leukaemia
cells is due, in large part, to cell cycle arrest and apoptosis. The apoptotic effect of cockle
GAG on leukemia cell is consistent with the apoptotic effect of low concentrations of heparin
on the lymphoblast and the cell cycle arrest cause by cockle GAG may provide an insight to
the molecular mechanism of the apoptotic effect this novel GAGs.
235
4.8 Crude and purified whelk GAG extracts inhibit cancer cell growth by apoptosis,
analysis by annexin V staining
Apoptosis is characterised by cell shrinkage, condensation of the nuclear chromatin,
and fragmentation of the nucleus and the apoptotic bodies (Hoffbrand, 1998: Kroemer et al,
1997). The biochemical event that characterises apoptosis and appears to be related to the
nuclear condensation and fragmentation is double-stranded cleavage of DNA
internucleosomal sites (Koury, 1992: Arends et al, 1990).
Apoptosis is also characterised by membrane damaged, leading to a subsequent
leakages of the phosphotidylserine into the outer menbranes layers and Annexin V is a
recombinant phosphatidylserine-binding protein that binds strongly and specifically to
phosphatidylserine residues. Only the apoptotic cells are expected to stain positive for
annexin V-FITC at the early stage of apoptosis while the necrotic cells stain positive for PI.
However, at late apoptosis stage, the damaged cells are expected to stain positive for both PI
and annexin V-FITC stains because at late apoptosis, the cells can be killed via apoptotic or
necrotic pathway and distinguishing between the two processes may be difficult.
The work presented in this project has demonstrated that both crude and ion –
exchange purified whelk GAG extracts can induce time-dependent apoptosis on certain
cancer cell lines. Crude whelk GAG extracts induces time-dependent apoptosis on both breast
cancer cells (MDA468 and MDANQ01) and cervical cell (HeLa) as shown in Figure 3.17,
3.21 and 3.22. Interestingly, the apoptotic effect of crude whelk GAG mixture was more
pronounced on cervical cell with apoptotic cell population of about 50-70%. Consistently, the
purified fraction E induced mild but not statistically significant (P>0.05) late apoptosis and
necrosis effect on both MDANQ01 and MDA468 cells with time-dependent increase in the
number of late apoptotic cells in MDA468 cell. Concisely, DAPI Fluorescent microscopy
236
results also showed some cells with morphological changes that characterised late apoptosis
(Figure 3.18 and 3.22).These results are consistent with the findings of Wengers and other
researchers on low molecular weight GAGs and other GAGs mimetics. The work of Wengers
and others showed that low molecular weight heparin elicit their anticancer activities on
pancreatic cancer by apoptosis induction (Wenger et al 2009). Erduran and others have also
reported apoptotic effect of heparin on different human carcinoma and lymphoblast (see
section 4.7). The difference in pharmacological activities of low molecular weight GAGs and
the unmodified GAGs have been attributed to their enhanced bioavailability which facilitates
their uptake into the cells (Lindhardt et al 2004).
Conclusively, the apoptotic effect of whelk GAG mixture on the two mammalian cells
appears to be largely associated with cell cycle arrest, DNA fragmentation, and
externalization of phosphatidylserine lipids. The cell cycle arrest cause by these GAG
extracts and its purified fraction E can also provide a great insight into the molecular
mechanism of action of apoptotic effect of crude whelk and purified fraction E. Conversely, it
is worthwhile, to investigate the activation level of the apoptotic proteins (bcl-2 and bax) as
well as caspase 3, 8 and 9. This will provide more insight into the molecular mechanism of
apoptotic effects of this novel GAGs.
4.9 PAGE and size exclusion analysis of cockle GAG mixture
Size exclusion assay results shows that the crude cockle extracts contain different
GAG structures with varying chain sizes and ionic properties (COO- and SO3
-). Although the
peaks from the gel filtration analysis were not extensively studied in this present work, the
densitometry analysis of the cellulose acetate dot blotting assay classified the fractions into
two broad peak according to their sizes/charges. GAGs are negatively charged polymers
237
consist of repeating units of disaccharides containing one uronic acid or galactose and one N-
acetylglycosamine. The variation in charge may be very large since each disaccharide is more
or less sulfated. The ionic bonding between cationic dyes (Azure A) and the negatively
charged GAGs are generally thought to be proportional to the number of negative charges
present on the GAG chain i.e. both sulfate and carboxyl groups (stone et al, 1994). The azure
A dye was only bound to the sulfated polysaccharide because of the suitable arrangement of
GAG ionic sites for interactions with the dye dimer but was not found to bind with other
compounds including proteins (Samir and Kost 2000). Hence, the wells stained with azure A
dye in the present work suggest the presence of GAGs with varying concentrations and
different sulfation levels. Electrophoresis mobility of the cockle GAG samples on PAGE was
visualized with azure A staining.
Additionally, slight variations in mobilities between the crude and depolymerised
samples were also observed. Difference in electrophoretic mobility of the various intact GAG
chains is an indication of distinctive structures present within these polysaccharides
(Vijayabaskar and Somasundaram 2012). The GAG extracts isolated in this study was
compared with commercial GAGs (HS, CS/DS) (Figure 3.34&3.36) to initially determine the
typical chain lengths and general level of sulfation from the mollusc derived GAG samples.
Dietrich and other researchers showed that sulfated polysaccharide had different
electrophoretic mobilities for different buffer system, depending on the structure of the
polysaccharide (Mariana and Barbara 1999: Dietrich et al 1989). PAGE analysis results
supported the evidence that crude cockle extracts did indeed contain GAGs and the GAGs-
like compound isolated contained CS/DS and HS-like members of the GAG family.
However, the exact nature of the structural differences between typical commercially
available porcine HS, CS, DS and the mollusc derived GAGs remains to be determined. This
will be critical in determining the exact nature of the biological activity of the mollusc
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derived GAGs. it is assumed that there must be subtle structural differences in these GAG
chains that do not appear in the commercially available GAGs which did not show any
cellular toxicity on the cancer cell lines tested in this study. The bare minimum for
investigating structual differences in GAG chains is to perform a disaccharide analysis where
the GAG chains are chemically or enzymatically reduced to their constituant discaccharides
and then individually quantified by strong ion-exchange chromatography. This data will at
best only provide limited information on structure activity relationships attributed to these
GAGs. It will take many years to determine the exact nature of the GAG binding sequences
involved in these observed anti-cancer activities.
4.10 SAX-HPLC and gel-filtration of cockle GAG extracts
SAX-HPLC analysis of chondroitinase ABC lyase digest confirmed the presence of
three major disaccharide components in the crude cockle GAG mixture. The non-sulfated
disaccharide (ΔUA-GalAc) has the highest composition, in contrast to the commercial CS/DS
in which this disaccharide was absent. The two most abundant CS/DS mono-sulfated
disaccharides [ΔUA-GalNac (6S) and ΔUA-GalNac (4S)] were also present in in the same
proportion in the crude GAG mixture, whereas the commercial CS were found to contain
high level of ΔUA-GalNac (6S) and a low level of ΔUA-GalNac (4S) disaccharides. This
unique structural composition formed the major difference between the crude cockle CS and
the commercial CS GAGs.
This result also suggests that this crude GAG extracts contains less sulfated CS-like
GAGs: this slight structurer modification may in part contribute to it’s growth inhibitory
effect on leukaemia cells. Predictably, the anti-tumour activity of this crude GAG extracts
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may in part due to the unique structurer composition of its CS-like chain and the possible
explanation for this bioactivivity may be linked to the suggestion of Asimakopoulou and
coworkers in his comprehensive review on biological Role of Chondroitin Sulfate in Cancer
and Chondroitin-based Anticancer Agents. He suggested that the important roles play by this
GAG molecule in cancer biology may be attributed to their involvement in various
interactions with tumour cells and other effective molecules, such as growth factors and also
affects several signaling pathways (Asimakopoulou et al, 2008). He also stressed the need for
proper understanding of the biological role of CS in cancer, tumour angiogenesis and
invasion. This suggestion has favoured the development of novel drugs which target the
tumour cells and the interactions with other effective molecules of the ECM or the cell
surface (Asimakopoulou et al, 2008).
Similarly, Kozlowski and other groups have reported an isolation of dermatan sulfates
from S. plicata and P. Nigra. This DS was found to contain the same disaccharide core
structure [α-L-IdoA(2SO4)-1→3β-D-GalNAc]n, but sulfated at carbon 4 or 6 of the GalNAc
residues, respectively (Kozlowski and Pavao, 2011: Kozlowski et al., 2011). Both ascidian
dermatan sulfates regardless of the position of sulfation on the N-acetylgalactosamine
drastically attenuate metastasis of both MC-38 colon carcinoma and B16-BL6 melanoma
cells, and the infiltration of inflammatory cells in a thioglycollate peritonitis mouse model
(Kozlowski and Pavao, 2011; Kozlowski et al., 2011).
Pumphrey and co-workers has also reported similar role of a novel modified CS
molecule (neoglycans) on cancer cells. This molecule was found to reduce cell viability by
induction of apoptosis of myeloma and cancer cells in vitro. Pumphrey in his work also
reported that, EDAC-modified CS reduced or abolished tumour growth, when injected
directly into breast tumours growing in nude mice (Asimakopoulou et al, 2008: Borsig et al,
2007: Pumphrey et al, 2002).
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Several studies have reported the role of CS in promoting tumour growth and
mediating events that enhance tumour invasion and metastasis effects that can be abolished
by chemically modified CS, or the use of CS with altered sulfation patterns (Asimakopoulou
et al, 2008: Borsig et al, 2007: Pumphrey et al, 2002). Some of these studies have proved the
potential use of modified CS as a potent anti-cancer agent. Although the cockle derived CS
chains appear to have an unusual disaccharide composition in comparison to commercial
porcine CS, we cannot confirm absolutely that the link between these differences and the
anticancer activities seen in this study.
Moreover, differences in HS structure have already been implicated in this study as
being linked to the cockle GAG extracts anti-cancer activities. Structural studies of cockle
GAG extracts also implicated HS in the biological activity seen on cancer cells. Quantitative
and qualitative analysis of HS oligosaccharides mapping was performed by depolymerising
cockle GAG extracts with a mixture of Heparinase I, II and III and then analysing the
resulting unsaturated oligosaccharides by SAX-HPLC chromatography. The most important
differences seen between the commercial HS GAGs and cockle extracted HS-like GAG
chains is the absence of ∆UA (2S)-GlcNAc, disulfated ∆UA(2S)-GlcNAc(6S) and the tri-
sulfated ∆UA(2S)-GlcNS(6S). A very low level of ∆UA-GlcNS (6S) and ∆UA (2S)-GlcNS
was also observed in the crude GAG mixture.
Thus, these result suggests that cockle GAG mixture contain low sulfated HS-like
GAG with low 2 O sulfate group because of the absence of trisulfated ∆UA2S (1→4)
GlcNS6S and disulfated ∆UA2S (1→4) GlcNAc6S disaccharides. PAGE analysis and TSK
gel-filtration results confirmed the presence of HS-like disaccharides in the heparinase
digested cockle GAG extracts.
This is an extremely unusual disaccharide compositional analysis for HS. Many
studies have reported the isolation of HS-like GAGs with various disaccharides compositions
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from different molluscs. Dietrich and coworkers in their work isolated highly sulfated HS-
like GAGs from various molluscs, in contrast to the usual low sulfated HS-like GAGs that are
usually isolated from molluscs (Volpi and Maccari 2005: Kim et al 1998: Dietrich et al
1989). Vijayabaskar and other groups had previously reported an isolation of HS-like species
from molluscs (Vijayabaskar and Somasundaram, 2012: Cesaretti et al, 2004: Jordan et al,
1986 and Dietrich et al, 1985). Pejler et al also reported the isolation of HS-like GAGs
containing a large amount of GlcN (3-O-sulfate) disaccharide from clam molluscs. This
disaccharide unit is a unique marker for the antithrombin-binding region of heparin/HS
disaccharide and it showed a similar antithrombin activity with unfractionated heparin (Pejler
et al 1987). Chi and his co-workers in their work reported an isolation of HS with a unique
structure, containing IdoA (2-O-sulfate)-GlcNAc as its major repeating disaccharides
sequence (Acharan sulfate) from African giant snail (Chi et al 2006: Kim et al 2004). HS-like
GAGs with unique disaccharide units composed of of non- sulfated, 2-O-sulfated or 3-O-
sulfated GlcA as well as 2-N-sulfated and/or 6-O-sulfated GlcN has also been isolated from
the bivalve Nodipecten nodosus (Gomes et al 2010). Interestingly, none of the above HS-like
GAGs has been shown to have any anticancer activity.
In addition, Dreyfuss and co-workers recently reported an isolation of heparin
mimetics with low 2 O sulfate group (similar to what was observed in this study) from
shrimp. This HS structural mimetics was shown to have anti inflammatory and anti
angiogenesis activities. It was clearly shown that the biological activity of this heparinoid was
due to its ability to interact with angiogenic growth factors such as FGF-2. He also linked the
antiangiogenic effect of this novel GAG to the presence of low content of 2-O-sulfate groups
in the shrimp heparin like GAG which in a similar manner to the 2-O-desulfated-heparin,
could competitively inhibit the interaction between growth factors and cell surface HS
proteoglycans (Dreyfuss et al 2010). Unfortunately, Dreyfuss failed to investigate the
242
anticancer activity of this HS mimetics and this present study has critically investigated the
anticancer activity of this unique HS-like GAG from cockle. The presence of low 2 O sulfate
groups was also observed in the HS like GAG isolated from cockle GAG and this structural
modification may explain the anticancer activity of this unique GAG.
Furthermore, there was a decrease of the specific sulfatation in position 2 of the
glucuronic acid unit with a strong increase of the disaccharides bearing non-sulfated
glucuronic acid and glucosamine. This decrease may also in part contribute to the inhibitory
effect of cockle GAG mixture on leukaemia cells due to important role of 2-O-sulfated IdoA
in HS-binding to FGF-2 a known survival factor for leukaemia cells grown in culture (Liuzzo
and Moscatelli 1996). Walker and others had earlier reported that structurally defined
oligosaccharides from HS that are rich in IdoA (2S)-containing disaccharides bind strongly to
FGF-2 and that the affinity for FGF-2 increases with oligosaccharide length and IdoA (2S)
content (Walker et al, 1994: Ishihara et al, 1993: Maccarana et al, 1993: Habuchi et al, 1992
and Turnball et al, 1992).
The presence of 2-O-sulfated IdoA has also been reported to be required for the
promotion of the growth-factor’s mitogenic activity. It is also noteworthy that extracted
cockle HS-like GAGs might be competed with the endogenous HS GAGs in the binding of
growth factors such as FGF-2 or blocking specific interactions of the cancer growth factors
(e.g.FGFs) with their receptors resulting into cell growth inhibition. It has previously been
shown that GAG-based drugs elicit their pharmacological effect in several ways: by
activating (agonists) or inactivating (antagonists) protein-based receptors (e.g.FGF-2),
competing with endogenous GAGs and/or inhibiting GAG biosynthesis (Gandhi et al., 2010).
Intruingingly, there is evidently a role for FGF-2 in haematopoiesis and the K562
leukaemia cell line has previously been shown to express HSPG’s that bind strongly to
FGF-2, therefore, this may be involved in modulation of its biologic activities (Olwin and
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Rapraeger, 1992 : Flaumenhaft et al, 1982). HS is also necessary for the long-term biologic
activity of FGF-2, the presence of HSPGs in the K562 cell line could have significant effects
on the ability of these cells to respond to FGF-2 by promoting the formation of the FGF-
2/HS/TK-receptor ternary signalling complex, hence promoting cell growth (Liuzzo and
Moscatelli 1996).
Structural variations between K562 HS and cockle GAG HS may impinge on the
ability of FGF-2 to bind its TK cell surface receptors, thereby inhibiting cell proliferation and
functions, thus, this may manifest itself partly in the anticancer activities seen with cockle
GAGs on the K562 cell line.
Taken together, previous data discussed above and the results reported here strongly
suggest that the novel GAGs isolated from cockle is capable of sequestering the growth
factors, making them unavailable for the interaction with their receptors and thus inhibiting
tumour cell proliferations. Thus, the pharmacological and biochemical properties of cockle
GAG, such as anti cancer activity against leukemic cells with a very low IC50 point to this
compound as a compelling drug candidate for treating cancer disease.
4.11 Ion- exchange fractionation of crude whelk GAG mixture
The process of ion-exchange chromatography helped to enhance the activities of the
crude whelk GAG extract by removing the unwanted salt contaminant from the GAG
preparation (Saravanan et al, 2010). This partial purification of whelk GAG extracts has
allowed a better understanding of the structural compositions of these whelk derived GAG
chains. The ion-exchange chromatogram for crude whelk GAGs was shown in Figure 3.23.
GAG chain sub-populations were eluted as a number of well defined peaks ranging from 0.9-
3.0M NaCl gradient. Although, the fractions were not studied extensively in this project , in
244
terms of this exact structural composition, we did however identify from the chromatagram
the bioactive fraction E on DEAE column. This has proven to be very informative in
determining the active GAG family member in the whelk GAG extracts. It also suggested
that this fraction contained high charge density, high molecular weight and or high sulfated
polysaccharide chains based on its late elution position in the NaCl gradient.
This speculation was confirmed by the superose-12 size exclusion result, which
clearly showed fraction E to be comprises of very high molecular weight polysaccharide
chains (Figure. 3.42). Fraction E is similar in structural terms to the HS/ heparin-like fraction
isolated from other molluscs (Andrade et al, 2013:Vijayabaskar and Somasundaram, 2012:
Moses et al, 2002: Mariana and Barbara 1999). Although the anti-inflammatory,
anticoagulant and anti-angiogenic potentials of these HS-like GAGs isolated from molluscs
have been well documented, there is no information on their potential use as anti-cancer drug.
However, Giulianna and others were concentrating solely on the anticoagulant activity of this
fraction but failed to test the activity of this novel polysaccharide on cancer cells.
Interestingly, the result obtained in our study from the biological activity of this novel
fraction showed its important role in cancer cell death and this is certainly encouraging as a
platform for the future development of the whelk GAGs as an anti-cancer drug.
4.12 PAGE and size exclusion analysis of both crude and ion-exchange purified whelk
GAG extracts
PAGE analysis of both crude and purified whelk extracts confirmed them to be GAG-
like in nature. The electrophoresis mobility of both the crude and ion- exchange purified
fractions showed that they both contained different members of the GAGs family of
245
polysaccharides with different structural composition. Electrophoresis mobility of the sample
on PAGE was visualized with azure A staining.
There were notable differences in the electrophoretic mobility between intact samples
and enzyme/chemically depolymerised GAG samples as the depolymerised samples contain
smaller oligosaccharides that were capable of migrating faster than the crude sample. This
gives us a rapid means of determining the prescence of individual GAG family members such
as HS, CS and DS in extracts taken from mollusc tissue samples. The eletrophoretic mobility
of the crude GAG extracts also showed difference in mobilites when compared with
commercial porcine GAGs and this suggests a possible variation in both sulfate content and
average chain length of GAGs derived from both sources (see next section for further details)
Difference in electrophoretic mobility of the various GAGs is certainly an indication
of distinctive structures within these mollusc derived polysaccharides in comparison to the
porcine derived GAGs (HS,CS and DS) which showed no anti-cancer activities with the cell
lines tested in this study (Figures 3.34&3.36). Dietrich et al and Mariana and Barbara showed
that a sulfated polysaccharide had different electrophoretic mobility for different buffer
system, depending on the structure of the polysaccharide. Overall PAGE analysis results
supported the evidence that both crude and purified whelk GAG contain GAGs and the
GAGs-like compound isolated were CS/DS and HS-like GAGs.
Size exclusion assay results confirmed both crude and purified whelk fractions
contain different GAGs family members with widely varying sizes and ionic properties
(COO- and SO3
-). Although the fractions obtained from the superose-12 gel filtration
experiments were not extensively studied in the present work the densitometry analysis of
cellulose acetate dot blotting assay confirmed the presence of strongly anionic
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polysaccharides as a result of Azure A dye binding, which could be classified into five broad
peak according to their sizes.
GAGs are negatively charged (cationic) polymers consist of repeating units of
disaccharides containing one uronic acid or galactose and one N-acetylglycosamine. The
variation in charge may be very large since each disaccharide is more or less sulfated and
control of discaccharide composition is complex. The ionic bonding between charged dyes
such as Azure A and the negatively charged GAGs are generally thought to be proportional to
the number of negative charges present on the GAG chain, i.e., both sulfate and carboxyl
groups (stone et al, 1994).
The azure A dye was only bound to the sulfated polysaccharide because of the
suitable arrangement of GAG ionic sites for interactions with the dye dimer but was not
found to bind with other compounds including proteins (Samir and Kost 2001). Hence, the
dots stained with azure A dye in the present project work suggest the presence of GAGs with
varying concentration and different sulfation level seen in the crude GAG extracts.
4.13 SAX-HPLC and gel-filtration of whelk GAGs
The qualitative and quantitative analysis of chondroitinase ABC lyase depolymerised whelk
GAG mixture shows two distinct peaks when resolved by ion-exchnge chromatography and
their elution positions vary considerably from the commercial CS/DS GAGs
oligosaccharides. The two fractions B and C derived from anion-exchange chromatographic
analysis were the only two peaks from the ion exchange column that were sensitive to
chondroitinase-ABC enzymes and the resulting oligosaccharides mixtures resolved by SAX-
HPLC shows that fraction B contain non-sulfated ΔUA-GalNac as its major disaccharides
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peak and a low level of mono-sulfated ΔUA-GalNac(4S).This is significantly different to the
dissacharide composistion analysis seen with the commercial CS/DS. The disaccharides
composition of whelk fraction B is very similar to CS previously isolated from D.
melanogaster (Toyoda et al., 2000). Many other studies have reported isolation of CS/DS
with unique disaccharides compositions from invertebrates (Adamczyk et al 2010: Vilela-
Silva: Pavao et al 1998: Pavao et al 1995 ), however, the disaccharide compositions of these
invertebrates CS/DS are slightly different from whelk fraction B CS in terms of sulfation
pattern and level.
The whelk Fraction C peak matched the elution position of commercial CS/DS when
applied to the ion-exchange column which suggested a more traditional discaccharide
composition for this whelk GAG sub-fraction. This prediction for the disaccharide
composisition of whelk fraction C was confirmed by chondroitinase ABC lyase digestion
and the subsequent as resolved by SAX-HPLC showed two major disaccharides peaks eluted
at the same time with similar elution pattern to the commercial CS GAGs. Furthermore, crude
whelk GAG mixtures were also degraded by chondroitinase-ABC enzymes and the major
disaccharides peaks shown were ΔUA-GalNac6S and ΔUA-GalNac4S disaccharides. The
elution pattern and the retention time was also similar. It is notewhorthy that crude whelk
GAG mixtures and its purified fractions B and C contain low sulfated CS/DS disaccharides.
The CS disaccharides compositions of both crude and whelk fraction C is very
similar to the CS isolated from Ascidians by Xu et al. This GAGs has been reported to have
anti inflammatory activity, however, the author failed to investigate the anticancer activity of
this unique GAGs (Xu et al 2011). Although, most CS isolated from many invertebrates are
more sulfated than whelk CS and they are structurally different in terms of sulfation level and
pattern, hence, no anticancer activities has been reported for any of these GAGs (Adamczyk
et al 2010: Vilela-Silva: Pavao et al 1998: Pavao et al 1995). The structural differences
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between other invertebrates CS and whelk CS, couple with the low sulfation composition of
whelk CS may in part explain the anti cancer activity of this unique GAGs, more studies are
needed to substantiate this speculation.
4.14 SAX-HPLC and gel-filtration of whelk bioactive fraction E
Qualitative analysis of HS/Heparin GAGs contained in the purified whelk fraction E
was performed by depolymerisation with a mixture of heparinase’s I, II and III and with the
resulting unsaturated oligosaccharides analysed by SAX-HPLC. The whelk derived GAG
fraction E contains six oligosaccharides peaks in contrast to the commercial HS, which
contained eight standard disaccharides peaks. The major peak was assigned to non-sulfated
disaccharide ∆UA - GlcNAc. Other peaks were assigned to ∆UA-GlcNS, ∆UA-GlcNAc (6S),
∆UA-GlcNS(6S), ∆UA(2S) (1→4) GlcNAc(6S) and ∆UA(2S) GlcNS(6S) disaccharides
respectively. However, both ∆UA (2S)- GlcNAc and ∆UA(2S)GlcNS disaccharides were
completely absent in this polymer and this is the major difference between the novel fraction
E and the commercial GAGs.
Andrade et al in their recent work report an isolation of high sulfated HS/heparin
GAG from the crab G. Cruentata mollusc. They demonstrated that the crab HS/heparin GAGs
present intermediate structure between heparin and heparan sulfate. In addition, the crab
heparin-like is rich in 2-O-sulfated glucuronic acid residues, possesses low levels of
trisulfated disaccharides (∆UA (2S) GlcNS (6S) and lacks the defined pentasaccharide
structure related to the antithrombin binding site (Andrade et al 2013). Brito et al in their
work also isolated another HS/heparin from the shrimp. The shrimp contains mainly blocks
of disulfated disaccharide units containing glucosamine N-sulfated/6-O-sulfated linked to
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glucuronic acid [∆UA-GlcNS (6S)]. Sulfated regions consisting of glucosamine N-sulfated
linked to iduronic acid 2-O-sulfated (∆UA (2S) GlcNS) are also present (Brito et al 2008). A
recent work of Brito and co-workers also reported the isolation of another novel GAG with
different HS/heparin like structure from shrimp head L. vannamei . The novel GAG from
shrimp head possesses a high degree of N,6-sulfation and minor N-acetylation together with
the high content of glucuronic acid and an absence of non-sulfated iduronic acid (Brito et al
2014).
These researches show that HS/heparin with unique disaccharides entity are isolated
from different molluscs and the presence of high percentage of non sulfated disaccharide∆UA
- GlcNAc (60%) suggests that this GAG is more of HS like. The presence of disulfated
disaccharide ∆UA-GlcNS(6S), ∆UA(2S) (1→4) GlcNAc(6S) in whelk Fraction E is
consistent with the findings of Andrade and other research groups who have isolated these
disaccharides from other mollusc. However, most of the GAGs isolated from GAG molluscs
described by these researchers are more sulfated than whelk fraction E GAG.
Moreover, the absence of both ∆UA (2S)- GlcNAc and ∆UA(2S)GlcNS discaccharides in
whelk purified fraction E is extremely interesting as normally they would represent some of
the major disaccharide species associated with HS derived from cells and tissues.
These major differences between whelk purified fraction E, commercial HS and other
HS/heparin like GAGs from molluscs may explain the anticancer activity of this unique GAG
extract. In addition, it is generally accepted that the binding of HS to FG-2 play a critical role
in the biological activities of HS. This binding occurs through N-sulfated glucosamine and 2-
O sulfated iduronic acid and fraction E HS GAG contains low composition of this sulfation
motif. This finding and complete absence of ∆UA (2S)- GlcNAc and ∆UA(2S)GlcNS
disaccharides in whelk fraction E oligosaccharides composition may potentiate its
antiproliferative activity on MDA468 and MDANQ01 breast cancer cells. The fraction E HS
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is a structural heparin/HS, and thus it could interfere with the binding and cellular modulation
of many proangiogenic growth factors. It may also predictably block the specific interaction
with FGF to its tyrosine kinase receptor (Fearo et al 2007), thereby impede the dimerisation
of the FGFR receptor and ultimately block signalling process that leads to proliferation.
Similarly, the tri sulfated disaccharide ∆UA2S (1→4) GlcNS6S composition was
significantly low in the whelk fraction E HS–like GAGs (table 6). This result suggest that
whelk fraction E contain low sulfated HS like due to the low composition of the trisulfated
disaccharides in contrasts with data obtained for heparin, where about 80% all of
disaccharides are the ∆UA2S (1→4) GlcNS6S (Zhang et al 2009: Linhardt, 2009: Dietrichet
al., 1998). This result is also consistent with the work of Andrade et al on shrimp GAG.
Bivalve Anodonta anodonta (Andrade et al 2013).
TSK gel-filtration results also confirmed the presence of HS-like disaccharides (dp2)
in fraction E GAG. This result corroborates the findings of Andrade and co-workers who had
previously reported the isolation of HS-like disaccharides from different molluscs (Andrade
et al, 2013:Vijayabaskar and Somasundaram 2012: Brito et al 2008: Moses et al, 2000:
Mariana and Barbara 1999). Brito et al also report the isolation of HS GAG with low content
of 2-O-sulfate groups in the shrimp heparinoid. They suggest that the anti-angiogenic effect
of this GAG may be due to the presence of this unique disaccharide composition. Possibly
this compound, like the 2-O-desulfated-heparin, could competitively inhibit the interaction
between growth factors and cell surface HS proteoglycans (Brito 2008). In contrast to this
result, Volpi and co-workers reported the isolation of high sulfated HS/heparin like GAG
from large fresh water mollusc Bivalve Anodonta anodonta (Volpi 2005). The heparin/HS
from Anodonta Anodonta show a degree of sulfation similar to that of bovine mucosa heparin
because of the presence of similar percentage composition of trisulfated ∆UA2S (1→4)
GlcNS6S. It also contains a slight modification of other oligosaccharides and a significant
251
amount of disaccharides bearing the sulfation group at position 3 of the N-sulfoglucosamine -
6- sulfate. Its anticoagulant activity was also similar to that of bovine.
Other researchers have also reported an isolation of low sulfated HS that composed of
blocks of low sulfated GlcNAc containing disaccharides and also highly sulfated Glc2S-
containing disaccharides (Yamada et al 2011) from molluscs. Chi et al also report the
isolation of HS preparation with a unique structure from the giant African snail Achatina
fulica and named acharan sulfate. The major repeating disaccharide sequence in acharan
sulfate is IdoA (2-O-sulfate)-GlcNAc. Gomes et al in their recent work isolated a unique HS
from the bivalve Nodipecten nodosus (Linnaeus 1758). The disaccharide units in the HS
chain are composed of nonsulfated, 2-O-sulfated or 3-O-sulfated GlcA as well as 2-N-
sulfated and/or 6-O-sulfated GlcN, and the anticoagulant activity of the mollusk HS was 5-
fold lower than that of porcine heparin.
Interestingly, some of these HS-like GAGs isolated from other molluscs had
anticoagulant activities similar to mammalian heparin GAGs (Andrade et al,
2013:Vijayabaskar and Somasundaram 2012 and Moisés et al, 2000). However, none of these
studies reported anti-cancer activity associated with any of these HS-like GAGs isolated from
molluscs.
The results obtained so far show that fraction E contains HS-like GAG and this may
in part be associated with its biological activities seen in the present work. Many studies have
shown the anti proliferative effects of heparin GAG, low molecular weight heparin, ultra low
molecular weight heparin and some HS mimetics on different cells including lymphoblast,
VSMC and tumour cell (Erduran et al 2007: Erduran et al 2004:Patel et al 2002: Fedarko et al
1989: Castllot et al 1985). Erduran and other research groups investigated the mechanism of
antiproliferative effect of heparin. They reported the antiproliferative effect of heparin was
due to apoptosis and cell cycle arrest (Aksoy et al 2008: Erduran et al 2007). Heparin is a
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well established GAG with many therapeutic functions including antimetastatic and
antiproliferative effects.The biological roles of this GAG is structurally related to its ability to
bind growth factors including FGF-2 (Neha et al 2010). It is note worthy that the biological
activities of HSGAGs are due in large part to its structural composition and thereby modulate
the ability of many growth factors in their binding to their receptors. The present study
demonstrated that whelk purified fraction E contain low sulfated HS-like GAG with complete
absent of both ∆UA (2S)- GlcNAc and ∆UA(2S)GlcNS discaccharides. This unique
structural composition of whelk novel GAG provide an insight into its antiproliferative
activities against the breast cancer cells investigated in this study (see above discussion). The
anti-cancer activity of whelk fraction E HS-like GAG is a new and unique finding in
glycosaminoglycans study.
It is well known that HS binds and modulates the activities of heparin-binding growth factors
and their receptors, such as FGF’s which in turn control various aspects of tumour growth
and angiogenesis (Dreyfuss et al, 2010). Binding of growth factors to its tyrosine kinase
receptors causes dimerization and autophosphorylation/transphosphorylation of the receptors
which in turn triggers activation of the cytosolic tyrosine kinase, which targets specific
substrates for tyrosine phosphorylation. However, the purified whelk fraction E is structurally
similar to HS GAGs and can selectively inhibit several growth factors or proteins involved in
the above process and ultimately inhibit the tumour growth as observed in the present study.
Early studies have shown that heparin inhibits the phosphorylation of numerous signaling
pathways involved in proliferation and survival, such as mitogen activated protein kinase
(MAPK), protein kinase C (PKC) and casein kinase II (CKII) (Ottlinger et al 1993:Pukac et
al 1992: Castellot et al 1989 and Hathaway et al 1980).
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However the exact mode of action by which the whelk fraction E kills cancerous cells, at the
GAG structural level and determination of the cellular pathways involved, needs further
study.
We shouldn’t forget that heparinase degradation of both crude whelk and its purified
fraction E GAG extracts showed abolition of the anti-cancer activities seen with both breast
cancer cell lines in this study (Figures 3.13). Also complete degradation of fraction E by
heparinase III lyase confirmed this purified fraction is HS-like: hence implicating HS as the
contributor to the biological activities seen in this study. Further work needs to be undertaken
to confirm that the anti-cancer activity seen with the whelk GAGs and the cancer cells lines is
directly related to the presence of an unusual type of HS like GAG species.
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4.15 Overall summary
It is clear that the original aims and objectives of this study have been both met and
suppassed. The study has demonstrated that both shellfish utilised contain GAG-like
compounds, which were revealed experimentally to be CS/DS-like and HS-like GAGs. Anti-
cancer activity of GAGs from molluscs is reported for the first time in this study. Mollusc
GAGs have always been evaluated for anticoagulants and anti-inflammatory activities due to
the presence of HS/Heparin-like structure in its composition. The anti-cancer activities of
both molluscs studied were shown to be specific to certain cancer cells and this can also be a
tool in the future development of both mollusc GAGs into anti-cancer drugs. The low and
different IC50 recorded for the two novel GAGs on certain cancer cell lines make these
polysaccharide a candidate anti-cancer drugs to be developed in the future.
It is possible for the first time to study the mechanism of anti-tumour activity of both
novel GAGs using annexin V-FITC, DAPI fluorescence microscopy and flow cytometry, in
contrast to the conventional antiangiogenesis inhibiton, P-selectin inhibition and L-selectin
inhibition analyses that are commonly used to assess anti tumour activity of GAGs related
drugs. The problem encountered with the false positive apoptosis results observed with
annexin V-FITC assay was finally resolved by DAPI fluorescence microscopy and this made
the apoptotic data more concise and convincing. Fractionations of whelk GAGs have enabled
new insight into the heterogeneity nature of both CS/DS and HS-like GAGs in this molluscs.
Enzyme depolymerisations of the two crude polysaccharides confirm the presence of
different GAGs (CS/DS-like and HS-like GAGs) in their tissue. SAX-HPLC analysis of the
resulting oligosaccharides from the enzyme depolymerised samples gave insight into the
structural heterogeneity of different CS/DS and HS-like GAGs in the two molluscs. The
structural diversity of mollusc GAGs are reportedly even greater than that of vertebrate
255
GAGs (Andrade et al, 2013). The compositional analysis of both CS/DS and HS-like
disaccharides of the two shellfish and the commercial GAGs performed for the purposes of
this study provide insight into the sulfation level of each disaccharide in the total GAG
compositions. This made the structure comparism easy and the differences between the novel
and commercial GAGs were clearly seen. This study reveals that the biological activities of
these two polysaccharides are due largely to the presence of GAG-like compounds within
their composition. The depolymerised samples did not demonstrate any anti-cancer activities
in any of the cancer cells tested. Similarly, the two novel polysaccharides are revealed as
non-toxic to normal fibroblast cells; this will make it a better anti-cancer drug with a less
toxic effect. Finally, at this juncture, it is difficult to reach a concrete conclusion on the
mechanisms of apoptosis and cell cycle arrest, signaling pathways involved in tumour
growth, and more detailed structural elucidations of the two novel polysaccharides; therefore,
further research is required in this specific area.
Limitation of this study
This study was limited to isolation of GAGs from whelk and cockle from shell fish.
Also the anticancer activities evaluated were limited to MDA468, MDANQ01, K562,
MOLT-4, and HeLa cell lines. The cytotoxic effect of the two shell fish was only assessed on
3T3 normal fibroblast cell line.
Characterisation of the major components of the novel GAGs extracted from the two shell
fish was only done by conventional enzymatic and chemical method of analysis; the resulting
disaccharides composition were analysed by PAGE and SAX-HPLC.
256
Future Direction
There is need for more in-depth works on all aspect of this work, most importantly;
The anticancer activities of the two novel GAGs need to be investigated on other cancer cell
lines e.g MCF-7, T-47D, HL-60, MOLT-3.
The anticancer activities should also be assessed on primary tumour cell
In vivo study is also highly essential for the anticancer evaluation of these novel GAGs
The cytotoxic effects can also be investigated on more normal, non cancerous cell line e.g.
MCF-12, MCF-17, HUVEC and other normal epithelial cell lines.
There is need to study the various signalling pathways involved in proliferation e.g MAPK,
MEK, ERK. The effect of the novel GAGs on cell cycle regulators e.g cyclin A, B,D and E,
CDKI,CDK2, CDK 4 e.t.c needs to be investigated.
Apoptosis signalling pathway e.g. caspace 3, 8 and 9, bcl-2, bax e.t.c. should also be
investigated before and after treatment with the novel GAGs.
Structural and compositional analysis of the major biological components of the two novel
GAGs can also be studied by MS-LC, FACE, NMR e.tc.
257
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